CA3141712A1 - Gene therapy for alzheimer's disease - Google Patents

Abstract

The present disclosure provides, among other things, human codon-optimized sequences encoding presenilin 1, and methods for using the sequences in gene therapy to treat neurodegenerative diseases including, but not limited to Alzheimer's disease, frontotemporal dementia, frontotemporal lobar degeneration, Pick's disease, Lewy body dementia, memory loss, and cognitive impairment including mild cognitive impairment (MCI).

Description

2 PC

GENE THERAPY FOR ALZHEIMER'S DISEASE
CLAIM OF PRIORITY
This application claims the benefit of U.S. Provisional Patent Application Serial No.
62/852,716, filed on May 24, 2019. The entire contents of the foregoing are hereby incorporated by reference.
FEDERALLY SPONSORED RESEARCH OR DEVELOPMENT
This invention was made with Government support under Grant No. NS041783 awarded by the National Institutes of Health. The Government has certain rights to the invention.
TECHNICAL FIELD
Described herein are, inter al/a, compositions and methods for using presenilin genetic therapy constructs to treat Alzheimer's disease (AD) and other neurodegenerative diseases.
BACKGROUND
Alzheimer's disease, also known as Alzheimer disease, accounts for majority of neurodegenerative dementia and is the fourth leading cause of death in the United States after heart disease, cancer and stroke. It is characterized by a progressive loss of cognitive function, neurodegeneration, neurofibrillary tangles and amyloid plaques in the brains of patients. Although the progression speed varies in different patients, the average life expectancy following diagnosis is three to nine years. Currently, there is no treatment for Alzheimer's disease.
SUMMARY
Described herein are methods and compositions that can be used to treat subjects with Alzheimer's disease (AD) and other neurodegenerative diseases, disorders or conditions. The present disclosure is based, at least in part, on the discovery that providing a codon-optimized wild-type PSEN1 cDNA into cells carrying heterozygous or homozygous dominant negative Psenl mutations, a well-established familial Alzheimer's disease model, provided unexpectedly high expression levels and rescued the impaired y-secretase activity in these cells. Thus, the present disclosure provides methods for effective gene therapy based on PSEN1 (to express PS1) and/or PSEN2 (to express PS2) for Alzheimer's disease and other neurodegenerative dementia, representing a significant breakthrough in this disease area.
Provided herein are compositions comprising a human codon-optimized polynucleotide encoding a human presenilin 1 protein (PS1), e.g., a polynucleotide comprising SEQ ID NO:9 or a sequence that is at least 80%, 90%, 95%, or 99%
identical to SEQ ID NO:9 (with at least one codon optimized with respect to wild type).
Exemplary human PS1 protein sequences include SEQ ID NOs:5 and 6, and can include sequences that are at least comprising a human codon-optimized polynucleotide encoding a human presenilin 1 (PSEN1) thereto. In some embodiments, the composition is associated with (e.g., formulated for delivery using) an exosome or lipid-based nanoparticle (LNP).
Also provided herein are compositions comprising a vector for expression of human PSEN1 in a cell, comprising a human codon-optimized polynucleotide described herein, operably linked to a promoter.
Also provided herein is the use of any of the compositions described herein in a method o treating a neurodegenerative disease, disorder, or condition in a subject.
In some embodiments, the vector is a viral vector, e.g., an adeno-associated viral (AAV) vector (such as AAV9 or AAVrh10); a lentiviral vector; or a retroviral vector.
In some embodiments, the promoter is a pan neuronal promoter, e.g., a synapsin I
promoter, or a neuron subtype-specific promoter, e.g., an alpha-calcium/calmodulin kinase .. 2A promoter.
Also provided herein are methods for treating a neurodegenerative disease, disorder, or condition, the method comprising administering to a human subject in need of treatment a composition described herein , wherein the subject has one or more mutations in at least one allele of PSEN1, preferably a mutation that encodes a dominant negative PSEN1 protein isoform.
In some embodiments, the neurodegenerative disease, disorder or condition is Alzheimer's disease.
In some embodiments, the Alzheimer's disease is familial Alzheimer's disease.
In some embodiments, the Alzheimer's disease is late-onset Alzheimer's disease.
In some .. embodiments, the Alzheimer's disease is sporadic Alzheimer's disease. In some embodiments, the Alzheimer's disease is early-onset Alzheimer's disease.
In some embodiments, the subject has a mutation at E280, Y115, L166, C410, Aex9, G548, D257, R278, L435, G384, L392, N141, G206, H163, A79, S290, A260, A426, A431, R269, L271, C1410, E280, P264, E185, L235, M146, e.g., a E280A, Y115H, L166P, C410Y, Aex9, G548, D257A, R278I, L435F, G384A, or L392V mutation in the PSEN1 gene, or a N141I, G206A, H163R, A79V, S290C, A260P, A426P, A431E, R269H, L271V, C1410Y, E280G, P264L, E185D, L235V, or M146V mutation in the PSEN1 gene.
In some embodiments, the neurodegenerative disease, disorder or condition is frontotemporal dementia, memory loss, cognitive decline or impairment. In some embodiments, the cognitive impairment is mild cognitive impairment (MCI).
In some embodiments, the composition is administered to the CNS of the subject in need of treatment.
In some embodiments, the polynucleotide encoding PSEN1 and/or PSEN2 gene or mRNA is administered to the CNS via intravenous delivery, via intrathecal delivery, via intracisternal delivery, via intracerebroventricular delivery, or via stereotactic injection into certain areas of the brain, optionally into the cerebral ventricles, or via direct injection into hippocampus or cortical areas Unless otherwise defined, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. Methods and materials are described herein for use in the present invention; other, suitable methods and materials known in the art can also be used. The materials, methods, and examples are illustrative only and not intended to be limiting. All publications, patent applications, patents, sequences, database entries, and other references mentioned herein are incorporated by reference in their entirety. In case of conflict, the present specification, including definitions, will control.
Other features and advantages of the invention will be apparent from the following detailed description and figures, and from the claims.
DESCRIPTION OF DRAWINGS
FIGs. IA-B. Introduction of WT hPS1 rescues impaired y-secretase activity in mutant MEFs. A, y-Secretase activity measured by NICD production is reduced in mutant MEF cells in a PS dosage dependent manner (WT > PS1 heterozygous KI or KO > homozygous or KO > DKO). B, Restoring impaired y-secretase activity by WT hPS1.
Increasing amounts of pCI-hPSEN1 plasmid DNA, as indicated, are transfected into MEFs of varying genotypes.
Western analysis showed that both PS1 NTF and NICD are restored in various PS
mutant MEFs. Heterozygous L435F KI cells are labeled as KI/+ or PS1L435F/+. N=3 independent experiments. Data represent mean SEM. *p <0.05; **p < 0.01; ***p < 0.001 (one-way ANOVA with Tukey's post-hoc analysis).

3 FIG 2. Sequence comparison of the endogenous human PSEN1 (hPSEN1) cDNA and the codon optimized hPSEN1 cDNA (Opti-hPSEN1) FIGs. 3A-B. Increased expression levels of PS1 NTF with codon optimized PSEN1 cDNA. A, Psen-null MEFs were transfected with increasing amounts of plasmids expressingexpressing the wild-type endogenous hPSEN1 cDNA (wt PS1) or the codon optimized hPSEN1 cDNA (opti PS1), and Western analysis was carried out using an antibody specific for PS1 N terminus. Untrans: untransfected MEFs as negative control. B, Quantification of PS1 NTF levels in cells transfected with either wild-type endogenous hPSEN1 cDNA (wt PS1) or the codon optimized hPSEN1 cDNA (opti PS1). Data are .. expressed as Mean SEM (n=3 independent experiments) FIG. 4. Codon optimization led to increased y-secretase activity. PS DKO MEFs were transfected with increasing amounts (12.5, 25, 50 or 100 ng) of pCI-hPS1 or pCI-hPSlopti plasmid DNA and CMV-NAE followed by Western analysis of NICD. MEFs that were untransfected or transfected with the empty vector were included as negative controls. We found that pCI-hPSlopti led to significantly higher levels of y-secretase activity, measured by NICD production, relative to pCI-hPS1. Data are expressed as mean SEM (n=5 independent experiments). Two-way ANOVA was used to assess statistical significance. **p <0.01.
DEFINITIONS
In order for the present disclosure to be more readily understood, certain terms are first defined below. Additional definitions for the following terms and other terms are set forth throughout the specification.
Administration:
As used herein, the term "administration" refers to the delivery or application of a composition to a subject or system. Administration to an animal subject (e.g., to a human) may be by any appropriate route. For example, in some embodiments, administration may be bronchial (including by bronchial instillation), buccal, enteral, intra-arterial, intradermal, intragastric, intramedullary, intramuscular, intranasal, intraperitoneal, intrathecal, intravenous, intraventricular, mucosal, nasal, oral, rectal, subcutaneous, sublingual, topical, tracheal (including by intratracheal instillation), transdermal, vaginal and vitreal.

4 Biologically active:
As used herein, the phrase "biologically active" refers to a characteristic of any substance that has activity in a biological system (e.g., cell culture, organism, etc.). For instance, a substance that, when administered to an organism, has a biological effect on that organism, is considered to be biologically active. Biological activity can also be determined by in vitro assays (for example, in vitro enzymatic assays). In particular embodiments, where a protein or polypeptide is biologically active, a portion of that protein or polypeptide that shares at least one biological activity of the protein or polypeptide is typically referred to as a "biologically active" portion. In some embodiments, a protein is produced and/or purified from a cell culture system, which displays biologically activity when administered to a subject.
Control:
As used herein, the term "control" has its art-understood meaning of being a standard against which results are compared. Typically, controls are used to augment integrity in experiments by isolating variables in order to make a conclusion about such variables. In some embodiments, a control is a reaction or assay that is performed simultaneously with a test reaction or assay to provide a comparator. In one experiment, the "test"
(i.e., the variable being tested) is applied. In the second experiment, the "control," the variable being tested is not applied. In some embodiments, a control is a historical control (i.e., of a test or assay performed previously, or an amount or result that is previously known). In some embodiments, a control is or comprises a printed or otherwise saved record. A
control may be a positive control or a negative control. In some embodiments, the control may be a "reference control", which is a sample used for comparison with a test sample, to look for differences or for the purposes of characterization.
Gene Therapy:
As used herein, the term "gene therapy" refers to any treatment including the direct or indirect administration of a nucleic acid to a subject. In particular instances, a protein of therapeutic value is expressed from an administered nucleic acid.
Identity:
As used herein, the term "identity" refers to the overall relatedness between polymeric molecules, e.g., between nucleic acid molecules (e.g., DNA molecules and/or RNA
molecules) and/or between polypeptide molecules. Calculation of the percent identity of two nucleic acid sequences, for example, can be performed by aligning the two sequences for optimal comparison purposes (e.g., gaps can be introduced in one or both of a first and a

5 second nucleic acid sequences for optimal alignment and non-identical sequences can be disregarded for comparison purposes). In certain embodiments, the length of a sequence aligned for comparison purposes is at least 30%, at least 40%, at least 50%, at least 60%, at least 70%, at least 80%, at least 90%, at least 95%, or substantially 100% of the length of the reference sequence. The nucleotides at corresponding nucleotide positions are then compared. When a position in the first sequence is occupied by the same nucleotide as the corresponding position in the second sequence, then the molecules are identical at that position. The percent identity between the two sequences is a function of the number of identical positions shared by the sequences, taking into account the number of gaps, and the length of each gap, which needs to be introduced for optimal alignment of the two sequences.
The comparison of sequences and determination of percent identity between two sequences can be accomplished using a mathematical algorithm. For example, the percent identity between two nucleotide sequences can be determined using the algorithm of Meyers and Miller (CABIOS, 1989, 4: 11-17), which has been incorporated into the ALIGN
program .. (version 2.0) using a PAM120 weight residue table, a gap length penalty of 12 and a gap penalty of 4. The percent identity between two nucleotide sequences can, alternatively, be determined using the GAP program in the GCG software package using an NWSgapdna.CMP matrix. Various other sequence alignment programs are available and can be used to determine sequence identity such as, for example, Clustal.
Improve, increase, or reduce:
As used herein, the terms "improve," "increase" or "reduce," or grammatical equivalents, indicate values that are relative to a baseline measurement, such as a measurement in the same individual prior to initiation of the treatment described herein, or a measurement in a control individual (or multiple control individuals) in the absence of the treatment described herein. A "control individual" is an individual afflicted with the same type and approximately the same severity of, e.g., Alzheimer's disease, as the individual being treated, who is about the same age as the individual being treated (to ensure that the stages of the disease in the treated individual and the control individual(s) are comparable).
Neurodegeneration:
As used herein, the term "neurodegeneration" means a process in which one or more neurons are damaged, decrease in function, become dysfunctional, and/or are lost by cell death. Neurodegeneration encompasses both rapid, gradual, and intermediate forms.
Accordingly, a neurodegenerative disease, condition, or symptom is one characterized in that the disease is typically associated with neuronal damage, and/or cell death.

6 Subject:
As used herein, the term "subject" refers to a human or any non-human animal (e.g., a mammal such as a mouse, rat, rabbit, dog, cat, cattle, swine, sheep, horse or primate). A
human includes pre- and post-natal forms. In many embodiments, a subject is a human being. A subject can be a patient, which refers to a human presenting to a medical provider for diagnosis or treatment of a disease. The term "subject" is used herein interchangeably with "individual" or "patient." A subject can be afflicted with or is susceptible to a disease or disorder but may or may not display symptoms of the disease or disorder.
Suffering from:
An individual who is "suffering from" a disease, disorder, and/or condition (e.g., Alzheimer's disease) has been diagnosed with or displays one or more symptoms of the disease, disorder, and/or condition.
Susceptible to:
An individual who is "susceptible to" a disease, disorder, and/or condition has not been diagnosed with and/or may not exhibit symptoms of the disease, disorder, and/or condition. In some embodiments, an individual who is susceptible to a disease, disorder, and/or condition (for example, Alzheimer's disease) may be characterized by one or more of the following: (1) a genetic mutation associated with development of the disease, disorder, and/or condition; (2) a genetic polymorphism associated with development of the disease, disorder, and/or condition; (3) increased and/or decreased expression and/or activity of a protein associated with the disease, disorder, and/or condition; (4) habits and/or lifestyles associated with development of the disease, disorder, and/or condition; (5) a family history of the disease, disorder, and/or condition; (6) reaction to certain bacteria or viruses; (7) exposure to certain chemicals. In some embodiments, an individual who is susceptible to a disease, disorder, and/or condition will develop the disease, disorder, and/or condition. In some embodiments, an individual who is susceptible to a disease, disorder, and/or condition will not develop the disease, disorder, and/or condition.
Therapeutically effective amount:
As used herein, the term "therapeutically effective amount" refers to an amount of a therapeutic protein which confers a therapeutic effect on the treated subject, at a reasonable benefit/risk ratio applicable to any medical treatment. The therapeutic effect may be objective (i.e., measurable by some test or marker) or subjective (i.e., subject gives an indication of or feels an effect). In particular, the "therapeutically effective amount" refers to an amount of a therapeutic protein or composition effective to treat, ameliorate, or prevent a

7 desired disease or condition, or to exhibit a detectable therapeutic or preventative effect, such as by ameliorating symptoms associated with the disease, preventing or delaying the onset of the disease, and/or also lessening the severity or frequency of symptoms of the disease. A
therapeutically effective amount is commonly administered in a dosing regimen that may comprise multiple unit doses. For any particular therapeutic protein, a therapeutically effective amount (and/or an appropriate unit dose within an effective dosing regimen) may vary, for example, depending on route of administration, on combination with other pharmaceutical agents. Also, the specific therapeutically effective amount (and/or unit dose) for any particular patient may depend upon a variety of factors including the disorder being treated and the severity of the disorder; the activity of the specific pharmaceutical agent employed; the specific composition employed; the age, body weight, general health, sex and diet of the patient; the time of administration, route of administration, and/or rate of excretion or metabolism of the specific fusion protein employed; the duration of the treatment; and like factors as is well known in the medical arts.
Treatment:
As used herein, the term "treatment" (also "treat" or "treating"), in its broadest sense, refers to any administration of a substance (e.g., provided compositions) that partially or completely alleviates, ameliorates, relives, inhibits, delays onset of, reduces severity of, and/or reduces incidence of one or more symptoms, features, and/or causes of a particular disease, disorder, and/or condition. In some embodiments, such treatment may be administered to a subject who does not exhibit signs of the relevant disease, disorder and/or condition and/or of a subject who exhibits only early signs of the disease, disorder, and/or condition. Alternatively or additionally, in some embodiments, treatment may be administered to a subject who exhibits one or more established signs of the relevant disease, disorder and/or condition. In some embodiments, treatment may be of a subject who has been diagnosed as suffering from the relevant disease, disorder, and/or condition. In some embodiments, treatment may be of a subject known to have one or more susceptibility factors that are statistically correlated with increased risk of development of the relevant disease, disorder, and/or condition.
Although generally speaking "PS1" refers to the presenilin-1 protein, and "PS2"
refers to the presenilin-2 protein, in some cases PS1 or PS2 is used to refer to mRNA or gene.

8 DETAILED DESCRIPTION
The present disclosure provides, among other things, compositions and methods for treating subjects with Alzheimer's disease and other neurodegenerative diseases, disorders and conditions based on delivering functional presenilin-1 (PS1) protein to a subject in need thereof In particular, the present disclosure contemplates gene therapy by providing a human codon-optimized polynucleotide encoding a presenilin-1 (PS1) to a subject in need of treatment who has a PSEN1 or PSEN2 mutation, e.g., a dominant negative mutation, associated with AD, e.g., with early onset Familial Alzheimer's disease (FAD) or with late onset sporadic AD.
Various aspects of the invention are described in detail in the following sections. The use of sections is not meant to limit the invention. Each section can apply to any aspect of the invention. In this application, the use of "or" means "and/or" unless stated otherwise.
Methods of Treatment As non-limiting examples, the present methods include gene therapy to express wild-type human Presenilin-1 in a subject suffering from or susceptible to a neurodegenerative disease, e.g., associated with a dominant negative mutation in PSEN1 or PSEN2, e.g., Alzheimer's disease (e.g., familial AD patients carrying PSEN1 or PSEN2 mutations or sporadic AD patients). The objective of such a gene therapy is, among other things, to enhance expression of PS1 in the brains of familial or sporadic AD patients in order to correct or overcome a deficit in PS1 or PS2 expression and/or activity. In FAD
patients, it is expected that a gene therapy method described herein results in increased expression of wild-type PS1 in the brain, rescuing the impairment of y-secretase activity associated with PS1 or PS2 mutations.
Mutations in the Presenilin genes ¨ PSEN1 and PSEN2 ¨ are highly penetrant and account for ¨90% of all mutations identified in familial AD (FAD), highlighting their importance in the pathogenesis of AD. More than 260 distinct mutations in PSEN1 have been reported, and they are dominantly inherited and mostly missense mutations. It is known that dominant negative mutations in the PSEN1 and PSEN2 genes are associated with early onset familial Alzheimer's disease. It was generally believed that the PS1 and presenilin-2 (PS2) proteins are part of E -secretase complex, and that mutations in the PSEN1 and PSEN2 genes contribute to the accumulation of Amyloid beta (A13) protein in Alzheimer's disease patients. Pathogenic PSEN1 mutations act in cis to impair mutant PS1 function and act in trans to inhibit wild-type Presently-1 (PS1) function (Heilig et al. J
Neurosci 33:11606-717

9 (2013); Zhou et al. Proc Nat! Acad Sci USA 114:12731-12736 (2017). Typically, by their very nature, dominant negative mutations cannot be rescued by expression of wild type protein (Herskowitz, I. Nature, 329:219-222 (1987)). However, surprisingly, as shown herein, transfection of codon-optimized hPSEN1 cDNA into immortalized MEFs carrying heterozygous and homozygous PS1 mutations was able to rescue the impaired y-secretase activity in these cells even better than the wild-type human sequence (see Examples, below), indicating that expression of wild-type PS1 from a codon-optimized exogenous sequence can overcome the dominant negative effects of the mutant Presenilin protein.
Without wishing to be bound by any particular theory, expression of PS1 may accomplish this objective by increasing the total level of wild-type PS1, rescuing the impairment of y-secretase expression and/or activity in AD patients.
The methods and compositions described herein can equally be used to treat other neurodegenerative diseases, disorders or conditions.
Alzheimer's disease The methods described herein may be used to treat or reduce the risk of developing subjects with all types of Alzheimer's disease including, but not limited to, familial and sporadic Alzheimer's disease, early onset or late onset Alzheimer's disease.
In some embodiments, the present methods may be used to treat or reduce the risk of development of early onset familial form of Alzheimer's disease (AD) that is associated with mutations in presenilin-1 (PS1) and/or presenilin-2 (PS2) (Sherrington, et al., Nature 375:754-760 (1995);
Rogaev, et al., Nature 376:775-778 (1995); Levy-Lahad, et al., Science 269:970-973 (1995);
Hiltunen, et al., Eur. J. Hum. Genet. 8:259-266 (2000); Jonghe, et al., Hum.
Mol. Genet.
8:1529-1540 (1999); Tysoe, etal., Am. J. Hum. Genet. 62:70-76 (1998); Crook, etal., Nat.
Med. 4:452-455 (1998), all of which are incorporated by reference herein).
In some embodiments, the present methods may be used to treat a subject that has a mutation in the PSEN1 or PSEN2 allele, e.g., a mutation that has a dominant negative effect on wild-type PS proteins. Exemplary mutations include C410Y, Aex9, G548, D257A, L166P, R278I, L435F, G384A, Y115H, and L392V, as well as N141I, G206A, H163R, A79V, 5290C, A260P, A426P, A431E, R269H, L271V, C1410Y, E280G, P264L, E185D, L235V, and M146V mutations (see, e.g., Heilig etal., J. Neurosci., 33(28):11606-11617 (2013); Watanabe et al., J. Neurosci. 32(15):5085-5096 (2012); Brouwers et al., 2008 Ann Med 40 (8): 562-83); Watanabe and Shen, PNAS November 28, 2017 114 (48) 12635-12637; Zhou etal., PNAS November 28, 2017 114 (48) 12731-12736; Hsu etal., Alzheimers Res Ther.
2018 Jul 18;10(1):67). Additional exemplary mutations that may have a dominant negative effect on wild-type PS proteins can include, but are not limited to, in PSEN-1: N32N;
R35Q; D4Odel (delGAC); D4Odel (delACG); E69D; A79V; V82L; 183 M84del (DelIM, AI83/M84, AI83/AM84); I83T; M84V; L85P; P88L; V89L (G>T); V89L (G>C); C92S; V94M; V96F;
V97L; T99A; F105C; F105I; F105L; F105V; R108Q; L113 Ill4insT (Intron4, InsTAC, p.113+1delG, sp1ice5); L113P; L113Q; Y115C; Y115D; Y115H; T116I; T116N; T116R;

P117A; P117L; P117R; P1175; E120D (A>C); E120D (A>T); E120G; E120K; E123K;
Q127 R128del(CAGA);InsG(G) (c.379 382de1XXXXinsG); H131R; 5132A; Li 34R;
N135D; N1355; N135Y; A136G; M1391 (G>C); M1391 (G>A); M139K; M139L; M139T;
M139V; V142F; I143F; I143M; I143N; I143T; I143V; M1461 (G>C); M1461 (G>T);

(G>A); M146L (A>C); M146L (A>T); M146V; T1471; T147P; L150P; L153V; Y154C;
Y154N; Y156F; Y156 R157insIY; R1575; H163P; H163R; H163Y; A164V; W165C (G>C);
W165C (G>T); W165G; L166H; L166P; L166R; L166V; L166del; 1167del (TTAdel);
1167del (TATdel); I168T; 5169de1 (AS169, 5er169de1, A5170); 5169L; S169P;
5170F;
5170P; L171P; L173F (G>C); L173F (G>T); L173W; L174del; L174M; L174R; F1755;
F176L; F177L; F1775; S178P; G183V; E184D; E184G; V191A; 1202F; G206A; G206D;
G2065; G206V; G209A; G209E; G209R; G209V; 5212Y; 1213F; 1213L; I213T; H214D;
H214N; H214Y; G217D; G217R; L219F; L219P; L219R; R220P; Q222H; Q222P; Q222R;
Q223R; L226F; L226R; I229F; S230I; 5230N; 5230R; A231P; A231T; A231V; L232P;
M2331 (G>A); M2331 (G>C); M233L (A>T); M233L (A>C); M233T; M233V; L235P;
L235R; L235V; F237I; F237L; I238M; K239N; T245P; A246E; A246P; L248P; L248R;
L250F; L2505; L250V; Y2565; A260V; V261F; V261L; L262F; L262V; C263F; C263R;
P264L; G2665; P267A; P267L; P267S; R269G; R269H; L271V; V272A; E273A; E273G;
T274R; A275V; R278I; R278K; R2785; R278T; E280A; (Paisa); E280G; E280K; L282F;
L282R; L282V; F283L; P284L; P284S; A285V; L286P; L286V; T291A; T291P; K311R;
E318G; D333G; R352C; R352 5353insR; T354I; R358Q; 5365A; 5365Y; R377M; R377W;
G378E; G378V; G378fs; L381F; L381V; G384A; F386I; F3865; F388L; S390I; 5390N;
V391F; V391G; L392P; L392V; G394V; A396T; N4055; 1408T; A409T; C410Y; V412I;
I416T; G4175; L418F; L420R; L424F; L424H; L424R; L424V; A426P; A431E;
(Jalisco);
A431V; A434C; A434T; L435F; P436Q; P436S; I437V; I439S; I439V; T440del; 869-2A>G;
869-22 869-23ins18 (AE9, A9, deltaE9); 1238 K239insI; 5290C;T291 5319de1 (AE9Finn, A9Finn, A9); 5290C;T291 5319de1 (AE9, A9); 5290C;T291 5319de1 A>G (AE9, A9);
5290C;T291 5319del G>A (AE9, A9); 5290C;T291 5319de1 G>T (AE9, A9); or 5290W;5291 R377de1 (A9-10 , Delta9-10, p.Ser290 Arg377delinsTrp, g.73671948 73682054del) (mutations are named relative to Uniprot P49768.1/GenBank Ref No. NM 000021.4), and in PSEN-2,; T18M; R29H; G34S; R62C; R62H; P69A; R71W;
K82R; A85V; V101M; K115Efs*; T122P; T122R; P123L; E126fs; E126K; S130L; V139M;

N1411 (Volga German); N141Y; L143H; V1481; K161R; R163H; H169N; M174V; S175C;
G212V; V214L; Q228L; Y231C; I235F; A237V; L238F; L238P; M239I; M239V; A252T;
A258T; T301M; K306fs; P334A; P334R; P348L; A377V; V393M; T430M; or D439A
mutations are named relative to Uniprot P49810.1/GenBank Ref. No. NP
000438.2). See, e.g., Sun et al., Proc Natl Acad Sci USA. 2017;114:E476¨E485; Heilig et al., J
Neurosci.
2013 Jul 10; 33(28):11606-17; Zhou et al., PNAS November 28, 2017 114 (48) 12731-12736.
.. In some embodiments, the methods can include determining that a subject has such a mutation, e.g., using methods known in the art. In some embodiments, the subject has a mutation as described herein (e.g., is identified as having a mutation as described herein using methods known in the art), and optionally has a family history of AD
and/or one or more symptoms of AD, and the subject is treated using a method described herein. In some embodiments, the subject does not yet have full AD.
Typically, increasing forgetfulness or mild confusion are early symptoms of Alzheimer's disease. Gradually, cognitive impairment associated with Alzheimer's disease leads to memory loss, especially recent memories, disorientation and misinterpreting spatial relationships, difficulty in speaking, writing, thinking, reasoning, changes in personality and behavior resulting in depression, anxiety, social withdrawal, mood swings, distrust in others, irritability and aggressiveness, changes in sleeping habits, wandering, loss of inhibitions, delusions, and eventually death.
Other neurodegenerative diseases, disorders or conditions In addition to Alzheimer's disease, the present methods may be used to treat other neurodegenerative diseases, disorders or conditions, including frontotemporal dementia, various types of memory loss, cognitive impairment including but not limited to mild cognitive impairment (MCI), or other conditions associated with loss of PS1 or PS2, e.g., due to a mutation in PSEN1 or PSEN2, e.g., that creates a dominant negative isoform.
Codon-Optimized Presenilin-1 (PSEN1) A codon-optimized presenilin-1 (PSEN1-encoding polynucleotide suitable for use in the compositions and methods described herein can include a full length cDNA
or a portion or fragment thereof that encodes a protein retaining substantial gamma secretase activity of the wild-type protein, e.g., at least 50% of the gamma secretase activity, or at least 60, 70, 80, 90, or 95%, or more than 100%, of the activity of the wild-type protein determined by (e.g., in in vitro y-secretase assays including those described in the Examples section, see also Watanabe et al., J. Neurosci. 32(15):5085-5096 (2012)). In some embodiments, a suitable codon-optimized PSEN1 encodes a protein sequence that is at least 80%, 85%, 90%, 95%, 96%, 97%, 98%, 99%, or 100% identical to the full-length wild type PS1 or PS2 protein sequence, respectively. Exemplary wild type genomic, cDNA or protein sequences of human PSEN1/PS1 or PSEN2/PS2 are shown in Table 1 and Figures 4A-C and 5A-B. PS1 is normally cleaved into N- and C- terminal fragments that are the active form.
PS-1 is processed to give two fragments: an N-terminal 28 kDa fragment, and a C-terminal 18 kDa fragment; the principal endoproteolytic cleavage occurs at and near Met298 in the proximal portion of the large hydrophilic loop (Podlisny et al., Neurobiol Dis.
1997;3(4):325-37;
Marambaud et al., EMBO J. 2002 Apr 15;21(8):1948-56). Sequences comprising or encoding these cleaved forms can also be used in the methods and compositions described herein, e.g., .. encoding amino acids 1-291, 1-292, 1-293, 1-294, 1-295, 1-296, 1-297, 1-298, or 1-299 of SEQ ID NO:5 or a corresponding fragment of SEQ ID NO:6-8.
Table 1: GenBank Accession Nos.
Isoform mRNA Protein RefSeqGene NM 000021.3 NP 000012.1 presenilin-1 isoform 1-467 NG 007386.2 (SEQ ID NO:1) (SEQ ID NO:5) Range 4965 to NM 007318.2 NP 015557.2 presenilin-1 isoform 1-463 92221 (SEQ ID NO:2) (SEQ ID NO:6) NM 000447.2 NP 000438.2 presenilin-2 isoform 1 NG 007381.1 (SEQ ID NO:3) (SEQ ID NO:7) Range 5001 to NM 012486.2 NP 036618.2 presenilin-2 isoform 2 30532 (SEQ ID NO:4) (SEQ ID NO:8) >NM 000021.3 Homo sapiens presenilin 1 (PSEN1), transcript variant 1, mRNA (SEQ ID NO:1) AAATGACGACAACGGTGAGGGTTCTCGGGCGGGGCCTGGGACAGGCAGCTCCGGGGTCCGCGGTTTCACA
TCGGAAACAAAACAGCGGCTGGTCTGGAAGGAACCTGAGCTACGAGCCGCGGCGGCAGCGGGGCGGCGGG
GAAGCGTATACCTAATCTGGGAGCCTGCAAGTGACAACAGCCTTTGCGGTCCTTAGACAGCTTGGCCTGG
AGGAGAACACATGAAAGAAAGAACCTCAAGAGGCTTTGTTTTCTGTGAAACAGTATTTCTATACAGTTGC
TCCAATGACAGAGTTACCTGCACCGTTGTCCTACTTCCAGAATGCACAGATGTCTGAGGACAACCACCTG
AGCAATACTGTACGTAGCCAGAATGACAATAGAGAACGGCAGGAGCACAACGACAGACGGAGCCTTGGCC

ACCCT GAGCCAT TAT CTAAT GGACGACCCCAGGGTAACT CCCGGCAGGT GGT GGAGCAAGAT GAGGAAGA

AGAT GAGGAGCT GACAT T GAAATAT GGCGCCAAGCAT GT GAT CAT GCT CT T T GT CCCT GT
GACT CT CT GC
AT GGT GGT GGT CGT GGCTACCAT TAAGT CAGT CAGCT T T TATACCCGGAAGGAT GGGCAGCTAAT
CTATA
CCCCAT T CACAGAAGATACCGAGACT GT GGGCCAGAGAGCCCT GCACT CAAT T CT GAAT GCT GCCAT
CAT
GAT CAGT GT CAT T GT T GT CAT GACTAT CCT CCT GGT GGT T CT GTATAAATACAGGT
GCTATAAGGT CAT C
CAT GCCT GGCT TAT TATAT CAT CT CTAT T GT T GCT GT T CT T T T T T T CAT T CAT T
TACT T GGGGGAAGT GT
T TAAAACCTATAACGT T GCT GT GGACTACAT TACT GT T GCACT CCT GAT CT GGAAT T T T
GGT GT GGT GGG
AAT GAT T T CCAT T CACT GGAAAGGT CCACT T CGACT CCAGCAGGCATAT CT CAT TAT GAT
TAGT GCCCT C
AT GGCCCT GGT GT T TAT CAAGTACCT CCCT GAAT GGACT GCGT GGCT CAT CT T GGCT GT
GAT T T CAGTAT
AT GAT T TAGT GGCT GT T T T GT GT CCGAAAGGT CCACT T CGTAT GCT GGT T GAAACAGCT
CAGGAGAGAAA
T GAAACGCT T T T T CCAGCT CT CAT T TACT CCT CAACAAT GGT GT GGT T GGT GAATAT
GGCAGAAGGAGAC
CCGGAAGCT CAAAGGAGAGTAT CCAAAAAT T CCAAGTATAAT GCAGAAAGCACAGAAAGGGAGT CACAAG
ACACT GT T GCAGAGAAT GAT GAT GGCGGGT T CAGT GAGGAAT GGGAAGCCCAGAGGGACAGT CAT
CTAGG
GCCT CAT CGCT CTACACCT GAGT CACGAGCT GCT GT CCAGGAACT T T CCAGCAGTAT CCT CGCT
GGT GAA
GACCCAGAGGAAAGGGGAGTAAAACT T GGAT T GGGAGAT T T CAT T T T CTACAGT GT T CT GGT
T GGTAAAG
CCT CAGCAACAGCCAGT GGAGACT GGAACACAACCATAGCCT GT T T CGTAGCCATAT TAAT T GGT T
T GT G
CCT TACAT TAT TACT CCT T GCCAT T T T CAAGAAAGCAT T GCCAGCT CT T CCAAT CT CCAT
CACCT T T GGG
CT T GT T T T CTACT T T GCCACAGAT TAT CT T GTACAGCCT T T TAT GGACCAAT TAGCAT T
CCAT CAAT T T T
ATAT CTAGCATAT T T GCGGT TAGAAT CCCAT GGAT GT T T CT T CT T T GACTATAACAAAAT
CT GGGGAGGA
CAAAGGT GAT T T T CCT GT GT CCACAT CTAACAAAGT CAAGAT T CCCGGCT GGACT T T T
GCAGCT T CCT T C
CAAGT CT T C CT GAC CAC CT T GCACTAT T GGACT T T GGAAGGAGGT GC CTATAGAAAAC GAT
T T T GAACAT
ACT T CAT CGCAGT GGACT GT GT CCCT CGGT GCAGAAACTACCAGAT T T GAGGGACGAGGT
CAAGGAGATA
T GATAGGCCCGGAAGT T GCT GT GCCCCAT CAGCAGCT T GACGCGT GGT CACAGGACGAT T T CACT
GACAC
T GCGAACT CT CAGGACTACCGT TAC CAAGAGGT TAGGT GAAGT GGT T TAAAC CAAACGGAACT CT
T CAT C
T TAAACTACAC GT T GAAAAT CAACCCAATAAT T CT GTAT TAACT GAAT T CT GAACT T T T
CAGGAGGTACT
GT GAGGAAGAGCAGGCACCAGCAGCAGAAT GGGGAAT GGAGAGGT GGGCAGGGGT T CCAGCT T CCCT T
T G
AT T T T T T GCT GCAGACT CAT CCT T T T TAAAT GAGACT T GT T T T CCCCT CT CT T T
GAGT CAAGT CAAATAT
GTAGAT T GCCT T T GGCAAT T CT T CT T CT CAAGCACT GACACT CAT TACCGT CT GT GATT
GCCAT T T CT T C
CCAAGGCCAGT CT GAACCT GAGGT T GCT T TAT CCTAAAAGT T T TAACCT CAGGT T CCAAAT T
CAGTAAAT
T T T GGAAACAGTACAGCTAT T T CT CAT CAAT T CT CTAT CAT GT T GAAGT CAAAT T T
GGAT T T T CCAC CAA
AT T CT GAAT T T GTAGACATACT T GTACGCT CACT T GCCCCAGAT GCCT CCT CT GT CCT CAT
T CT T CT CT C
CCACACAAGCAGT CT T T T T CTACAGCCAGTAAGGCAGCT CT GT CGT GGTAGCAGAT GGT CCCAT
TAT T CT
AGGGT CT TACT CT T T GTAT GAT GAAAAGAAT GT GT TAT GAAT CGGT GCT GT CAGCCCT GCT
GT CAGACCT
T CT T CCACAGCAAAT GAGAT GTAT GCCCAAAGACGGTAGAAT TAAAGAAGAGTAAAAT GGCT GT T
GAAGC
ACT T T CT GT CCT GGTAT T T T GT T T T T GCT T T T GCCACACAGTAGCT CAGAAT T T
GAACAAATAGCCAAAA
GCT GGT GGT T GAT GAAT TAT GAACTAGT T GTAT CAACACAAAGCAAGAGT T GGGGAAAGCCATAT
T TAAC
T T GGT GAGCT GT GGGAGAACCT GGT GGCAGAAGGAGAACCAACT GCCAAGGGGAAAGAGAAGGGGCCT
CC
AGCAGCGAAGGGGATACAGT GAGCTAAT GAT GT CAAGGAGGAGT T T CAGGT TAT T CT CGT CAGCT
CCACA
AAT GGGT GCT T T GT GGT CT CT GCCCGCGT TACCT T T CCT CT CAAT GTACCT T T GT GT
GAACT GGGCAGT G
GAGGT GCCT GCT GCAGT TACCAT GGAGT T CAGGCT CT GGGCAGCT CAGT
CAGGCAAAACACACAAACAGC
CAT CAGCCT GT GT GGGCT CAGGGCACCT CT GGACAAAGGCT T GT GGGGCATAACCT T CT T
TACCACAGAG

AGCCCT TAGCTAT GCT GAT CAGACCGTAAGCGT T TAT GAGAAACT TAGT T T CCT CCT GT GGCT
GAGGAGG
GGCCAGCT T T T T CT T CT T T T GCCT GCT GT T T T CT CT CCCAAT CTAT GATAT GATAT
GACCT GGT T T GGGG
CT GT CT T T GGT GT T TAGAATAT T T GT T T T CT GT CCCAGGATAT T T CT
TATAAGAACCTAACT T CAAGAGT
AGT GT GCGAGTACT GAT CT GAAT T TAAAT TAAAAT T GGCT TATAT TAGGCAGT
CACAGACAGGAAAAATA
.. AGAGCTAT GCAAAGAAAGGGGGAT T TAAAGTAGTAGGT T CTAT CAT CT CAAT T CAT T T T T
T T CCAT GAAA
T CCCT T CT T CCAAGAT T CAT T CCCT CT CT CAGACAT GT GCTAGCAT GGGTAT TAT CAT T
GAGAAAGCACA
GCTACAGCAAAGCCACCT GAATAGCAAT T T GT GAT T GGAAGCAT T CT T GAGGGAT CCCTAAT
CTAGAGTA
AT T TAT T T GT GTAAGGAT CCCAAAT GT GT T GCACCT T T CAT GATACAT T T CT T CT CT
GAAGAGGGTACGT
GGGGT GT GT GTAT T TAAAT CCAT CCTAT GTAT TACT GAT T GT CCT GT GTAGAAAGAT
GGCAAT TAT T CT G
T CT CT T T CT CCAAGT T T GAGCCACAT CT CAGCCACAT T GT TAGACAGT GTACAGAGAACCTAT
CT T T CCT
T T T T T T T T T T T TAAAGGACAGGAT T T T GCT GT GT T GCCCAGGCTAGACT T GAACT
CCT GGGCT CAAGTAA
T CCACCT CAGCCT GAGTAGCT GAGAC TACAGCCCAT CT TAT T T CT T TAAAT CAT T CAT CT
CAGGCAGAGA
ACT T T T CCCT CAAACAT T CT T T T TAGAAT TAGT T CAGT CAT T CCTAAAACAT CCAAAT
GCTAGT CT T CCA
C CAT GAAAAATAGAT T GT CACT GGAAAGAACAGTAGCAAT T T CCATAAGGAT GT GCCT T CACT
CACACGG
GACAGGCGGT GGT TATAGAGT CGGGCAAAAC CAGCAGTAGAGTAT GAC CAGCCAAGCCAAT CT GCT
TAAT
AAAAAGAT GGAAGACAGTAAGGAAGGAAAGTAGCCAC TAAGAGT CT GAGT CT GACT GGGCTACAGAATAA
AG G GTAT T TAT GGACAGAAT GT CAT TACAT G C C TAT GGGAATACCAAT CATATTT
GGAAGATTT GCAGAT
T T T T T T T CAGAGAGGAAAGACT CACCT T CCT GT T T T T GGT T CT CAGTAGGT T CGT
GT GT GT T CCTAGAAT
CACAGCT CT GACT CCAAAT GACT CAAT T T CT CAAT TAGAAAAAGTAGAAGCT T T CTAAGCAACT
T GGAAG
AAAACAGT CATAAGTAAGCAAT T T GT T GAT T T TAC TACAGAAGCAACAAC T GAAGAGGCAGT GT
T T T TAC
T T T CAGACT CCGGGAT T CCCAT T CT GTAGT CT CT CT GCT T T TAAAAACCCT CCT T T T
GCAATAGAT GCCC
AAACAGAT GAT GT T TAT TACT T GT TAT T TAC GT GGC CT CAGACAGT GTAT GTAT T CT C
GATATAACT T GT
AGAGT GT GAAATATAAGT T TAAC TAC CAAATAAGGT CT CCCAGGGT TAGAT GACT GCGGGAAGCCT
T T GA
T CCCAACCCCCAAGGCT T T GTATAT T T GAT CAT T T GT GAT CTAACCCT GGAAGAAAAAGAGCT
CAGAAAC
CACTAT GAAAAAAT T T GT T CAGT GT T T T CT GT GT T CCCGTAGGT T CT GGAGT CT
GAGGAT GCAAAGAT GA
ATAAGATAAAT T CT CAGAAT GTAGT TATAAT CT CT T GT T T T CT GGTATAT GCCAT CT T T
CT T TAACT T CT
C TAAAATAT T GGGTAT T T GT CAAATAAC CACT T T TAACAGT TAC CAT TACT GAGGGCT
TATACAT T GGT G
T TATAAAAGT GACT T GAT T CAGAAAT CAAT CCAT T CAGTAAAGTACT CCT T CT CTAAAT T T
GCT GT TAT G
T CTATAAGGAACAGT T T GACCT GCCCT T CT CCT CACCT CCT CACCT GCCT T CCAACAT T
GAAT T T GGAAG
GAGACGTGAAAATTGGACATTTGGTTTTGCCCTTGGGCTGGAAACTATCATATAATCATAAGTTTGAGCC
TAGAAGT GAT CCT T GT GAT CT T CT CACCT CT T TAAAT T CCCACAACACAAGAGAT
TAAAAACAGAGGT T T
CAGCT CT T CATAGT GCGT T GT GAAAT GGCT GGCCAGAGT GTACCAACAAAGCT GT CAT CGGGCT
CACAGC
T CAGAGACAT CT GCAT GT GAT CAT CT GCATAGT CCT CT CCT CTAACGGGAAACACCT CAGAT T
T GCATAT
AAAAAAGCACCCT GGT GCT GAAAT GAACCCCT T T CT T GAACAT CAAAGCT GT CT CCCACAGCCT
T GGGCA
GCAGGGT GCCT CT TAGT GGAT GT GCT GGGT CCACCCT GAGCCCT GACAT GT GGT GGCAGCAT T
GCCAGT T
GGT CT GT GT GT CT GT GTAGCAGGGACGAT T T CCCAGAAAGCAAT T T T CCT T T T
GAAATACGTAAT T GT T G
AGACTAGGCAGT T T CAAAGT CAGCT GCATATAGTAGCAAGTACAGGACT GT CT T GT T T T T GGT
GT CCT T G
GAGGT GCT GGGGT GAGGGT T T CAGT GGGAT CAT T TACT CT CACAT GT T GT CT GCCT T CT
GCT T CT GT GGA
CACT GCT T T GTACT TAAT T CAGACAGACT GT GAATACACCT T T T T TATAAATACCT T T
CAAAT T CT T GGT
AAGATATAAT T T T GATAGCT GAT T GCAGAT T T T CT GTAT T T GT CAGAT TAATAAAGACT
GCAT GAAT C CA

>NM 007318.2 Homo sapiens presenilin 1 (PSEN1), transcript variant 2, mRNA (SEQ ID NO:2) AAATGACGACAACGGTGAGGGTTCTCGGGCGGGGCCTGGGACAGGCAGCTCCGGGGTCCGCGGTTTCACA
TCGGAAACAAAACAGCGGCTGGTCTGGAAGGAACCTGAGCTACGAGCCGCGGCGGCAGCGGGGCGGCGGG
GAAGCGTATACCTAATCTGGGAGCCTGCAAGTGACAACAGCCTTTGCGGTCCTTAGACAGCTTGGCCTGG
AGGAGAACACATGAAAGAAAGAACCTCAAGAGGCTTTGTTTTCTGTGAAACAGTATTTCTATACAGTTGC
T CCAAT GACAGAGT TACCT GCACCGT T GT CCTACT T CCAGAAT GCACAGAT GT CT
GAGGACAACCACCT G
AGCAATACTAATGACAATAGAGAACGGCAGGAGCACAACGACAGACGGAGCCTTGGCCACCCTGAGCCAT
TATCTAATGGACGACCCCAGGGTAACTCCCGGCAGGTGGTGGAGCAAGATGAGGAAGAAGATGAGGAGCT
GACATTGAAATATGGCGCCAAGCATGTGATCATGCTCTTTGTCCCTGTGACTCTCTGCATGGTGGTGGTC
GTGGCTACCATTAAGTCAGTCAGCTTTTATACCCGGAAGGATGGGCAGCTAATCTATACCCCATTCACAG
AAGATACCGAGACTGTGGGCCAGAGAGCCCTGCACTCAATTCTGAATGCTGCCATCATGATCAGTGTCAT
TGTTGTCATGACTATCCTCCTGGTGGTTCTGTATAAATACAGGTGCTATAAGGTCATCCATGCCTGGCTT
ATTATATCATCTCTATTGTTGCTGTTCTTTTTTTCATTCATTTACTTGGGGGAAGTGTTTAAAACCTATA
ACGTTGCTGTGGACTACATTACTGTTGCACTCCTGATCTGGAATTTTGGTGTGGTGGGAATGATTTCCAT
TCACTGGAAAGGTCCACTTCGACTCCAGCAGGCATATCTCATTATGATTAGTGCCCTCATGGCCCTGGTG
TTTATCAAGTACCTCCCTGAATGGACTGCGTGGCTCATCTTGGCTGTGATTTCAGTATATGATTTAGTGG
CTGTTTTGTGTCCGAAAGGTCCACTTCGTATGCTGGTTGAAACAGCTCAGGAGAGAAATGAAACGCTTTT
TCCAGCTCTCATTTACTCCTCAACAATGGTGTGGTTGGTGAATATGGCAGAAGGAGACCCGGAAGCTCAA
AGGAGAGTAT CCAAAAAT T CCAAGTATAAT GCAGAAAGCACAGAAAGGGAGT CACAAGACACT GT T GCAG

AGAATGATGATGGCGGGTTCAGTGAGGAATGGGAAGCCCAGAGGGACAGTCATCTAGGGCCTCATCGCTC
TACACCTGAGTCACGAGCTGCTGTCCAGGAACTTTCCAGCAGTATCCTCGCTGGTGAAGACCCAGAGGAA
AGGGGAGTAAAACTTGGATTGGGAGATTTCATTTTCTACAGTGTTCTGGTTGGTAAAGCCTCAGCAACAG
CCAGTGGAGACTGGAACACAACCATAGCCTGTTTCGTAGCCATATTAATTGGTTTGTGCCTTACATTATT
ACTCCTTGCCATTTTCAAGAAAGCATTGCCAGCTCTTCCAATCTCCATCACCTTTGGGCTTGTTTTCTAC
TTTGCCACAGATTATCTTGTACAGCCTTTTATGGACCAATTAGCATTCCATCAATTTTATATCTAGCATA
TTTGCGGTTAGAATCCCATGGATGTTTCTTCTTTGACTATAACAAAATCTGGGGAGGACAAAGGTGATTT
TCCTGTGTCCACATCTAACAAAGTCAAGATTCCCGGCTGGACTTTTGCAGCTTCCTTCCAAGTCTTCCTG
ACCACCTTGCACTATTGGACTTTGGAAGGAGGTGCCTATAGAAAACGATTTTGAACATACTTCATCGCAG
TGGACTGTGTCCCTCGGTGCAGAAACTACCAGATTTGAGGGACGAGGTCAAGGAGATATGATAGGCCCGG
AAGTTGCTGTGCCCCATCAGCAGCTTGACGCGTGGTCACAGGACGATTTCACTGACACTGCGAACTCTCA
GGACTACCGTTACCAAGAGGTTAGGTGAAGTGGTTTAAACCAAACGGAACTCTTCATCTTAAACTACACG
TTGAAAATCAACCCAATAATTCTGTATTAACTGAATTCTGAACTTTTCAGGAGGTACTGTGAGGAAGAGC
AGGCACCAGCAGCAGAATGGGGAATGGAGAGGTGGGCAGGGGTTCCAGCTTCCCTTTGATTTTTTGCTGC
AGACTCATCCTTTTTAAATGAGACTTGTTTTCCCCTCTCTTTGAGTCAAGTCAAATATGTAGATTGCCTT
TGGCAATTCTTCTTCTCAAGCACTGACACTCATTACCGTCTGTGATTGCCATTTCTTCCCAAGGCCAGTC
TGAACCTGAGGTTGCTTTATCCTAAAAGTTTTAACCTCAGGTTCCAAATTCAGTAAATTTTGGAAACAGT
ACAGCTATTTCTCATCAATTCTCTATCATGTTGAAGTCAAATTTGGATTTTCCACCAAATTCTGAATTTG
TAGACATACTTGTACGCTCACTTGCCCCAGATGCCTCCTCTGTCCTCATTCTTCTCTCCCACACAAGCAG
TCTTTTTCTACAGCCAGTAAGGCAGCTCTGTCGTGGTAGCAGATGGTCCCATTATTCTAGGGTCTTACTC

T T T GTAT GAT GAAAAGAAT GT GT TAT GAAT CGGT GCT GT CAGCCCT GCT GT CAGACCT T
CT T CCACAGCA
AAT GAGAT GTAT GCCCAAAGACGGTAGAAT TAAAGAAGAGTAAAAT GGCT GT T GAAGCACT T T CT
GT CCT
GGTAT T T T GT T T T T GCT T T T GCCACACAGTAGCT CAGAAT T T GAACAAATAGCCAAAAGCT
GGT GGT T GA
T GAAT TAT GAAC TAGT T GTAT CAACACAAAGCAAGAGT T GGGGAAAGCCATAT T TAACT T GGT
GAGCT GT
GGGAGAACCTGGTGGCAGAAGGAGAACCAACTGCCAAGGGGAAAGAGAAGGGGCCTCCAGCAGCGAAGGG
GATACAGT GAGCTAAT GAT GT CAAGGAGGAGT T T CAGGT TAT T CT CGT CAGCT CCACAAAT
GGGT GCT T T
GT GGT CT CT GCCCGCGT TACCT T T CCT CT CAAT GTACCT T T GT GT GAACT GGGCAGT
GGAGGT GCCT GCT
GCAGT TAC CAT GGAGT T CAGGCT CT GGGCAGCT CAGT CAGGCAAAACACACAAACAGCCAT CAGCCT
GT G
T GGGCT CAGGGCACCT CT GGACAAAGGCT T GT GGGGCATAACCT T CT T TACCACAGAGAGCCCT
TAGCTA
T GCT GAT CAGACCGTAAGCGT T TAT GAGAAACT TAGT T T CCT CCT GT GGCT
GAGGAGGGGCCAGCT T T T T
CT T CT T T T GCCT GCT GT T T T CT CT CCCAAT CTAT GATAT GATAT GACCT GGT T T
GGGGCT GT CT T T GGT G
T T TAGAATAT T T GT T T T CT GT CCCAGGATAT T T CT TATAAGAACCTAACT T CAAGAGTAGT
GT GCGAGTA
CT GAT CT GAAT T TAAAT TAAAAT T GGCT TATAT TAGGCAGT CACAGACAGGAAAAATAAGAGCTAT
GCAA
AGAAAGGGGGAT T TAAAGTAGTAGGT T CTAT CAT CT CAAT T CAT T T T T T T CCAT GAAAT
CCCT T CT T CCA
AGAT T CAT T CCCT CT CT CAGACAT GT GCTAGCAT GGGTAT TAT CAT T
GAGAAAGCACAGCTACAGCAAAG
CCACCT GAATAGCAAT T T GT GAT T GGAAGCAT T CT T GAGGGAT CCCTAAT CTAGAGTAAT T
TAT T T GT GT
AAGGAT CCCAAAT GT GT T GCACCT T T CAT GATACAT T T CT T CT CT GAAGAGGGTACGT
GGGGT GT GT GTA
T T TAAAT CCAT CCTAT GTAT TACT GATT GT CCT GT GTAGAAAGAT GGCAAT TAT T CT GT CT
CT T T CT CCA
AGT T T GAGCCACAT CT CAGCCACAT T GT TAGACAGT GTACAGAGAACCTAT CT T T CCT T T T
T T T T T T T T T
AAAGGACAGGAT T T T GCT GT GT T GCCCAGGCTAGACT T GAACT CCT GGGCT CAAGTAAT
CCACCT CAGCC
T GAGTAGCT GAGACTACAGCCCAT CT TAT T T CT T TAAAT CAT T CAT CT CAGGCAGAGAACT T
T T CCCT CA
AACAT T CT T T T TAGAAT TAGT T CAGT CAT T CCTAAAACAT CCAAAT GCTAGT CT T CCAC
CAT GAAAAATA
GAT T GT CACT GGAAAGAACAGTAGCAAT T T CCATAAGGAT GT GCCT T CACT
CACACGGGACAGGCGGT GG
T TATAGAGT CGGGCAAAAC CAGCAGTAGAGTAT GAC CAGCCAAGCCAAT CT GCT TAATAAAAAGAT
GGAA
GACAGTAAGGAAGGAAAGTAGCCAC TAAGAGT CT GAGT CT GACT GGGCTACAGAATAAAGGGTAT T TAT
G
GACAGAAT GT CAT TACAT GCCTAT GGGAATAC CAAT CATAT T T GGAAGAT T T GCAGAT T T T
T T T T CAGAG
AGGAAAGACT CACCT T CCT GT T T T T GGT T CT CAGTAGGT T CGT GT GT GT T CCTAGAAT
CACAGCT CT GAC
T CCAAAT GACT CAAT T T CT CAAT TAGAAAAAGTAGAAGCT T T CTAAGCAACT T
GGAAGAAAACAGT CATA
AGTAAGCAAT T T GT T GAT T T TAC TACAGAAGCAACAACT GAAGAGGCAGT GT T T T TACT T T
CAGACT CCG
GGAT T CCCAT T CT GTAGT CT CT CT GCT T T TAAAAACCCT CCT T T T GCAATAGAT
GCCCAAACAGAT GAT G
T T TAT TACT T GT TAT T TACGT GGCCT CAGACAGT GTAT GTAT T CT CGATATAACT T
GTAGAGT GT GAAAT
ATAAGT T TAACTACCAAATAAGGT CT CCCAGGGT TAGAT GACT GCGGGAAGCCT T T GAT
CCCAACCCCCA
AGGCT T T GTATAT T T GAT CAT T T GT GAT CTAACCCT GGAAGAAAAAGAGCT CAGAAAC CAC
TAT GAAAAA
AT T T GT T CAGT GT T T T CT GT GT T CCCGTAGGT T CT GGAGT CT GAGGAT GCAAAGAT
GAATAAGATAAAT T
CT CAGAAT GTAGT TATAAT CT CT T GT T T T CT GGTATAT GCCAT CT T T CT T TAACT T
CT CTAAAATAT T GG
GTAT T T GT CAAATAAC CACT T T TAACAGT TAC CAT TACT GAGGGCT TATACAT T GGT GT
TATAAAAGT GA
CT T GAT T CAGAAAT CAAT CCAT T CAGTAAAGTACT CCT T CT CTAAAT T T GCT GT TAT GT
CTATAAGGAAC
AGT T T GACCT GCCCT T CT CCT CACCT CCT CACCT GCCT T CCAACAT T GAAT T T
GGAAGGAGACGT GAAAA
T T GGACAT T T GGT T T T GCCCT T GGGCT GGAAACTAT CATATAAT CATAAGT T T
GAGCCTAGAAGT GAT CC
T T GT GAT CT T CT CACCT CT T TAAAT T CCCACAACACAAGAGAT TAAAAACAGAGGT T T
CAGCT CT T CATA
GT GCGT T GT GAAAT GGCT GGCCAGAGT GTACCAACAAAGCT GT CAT CGGGCT CACAGCT
CAGAGACAT CT

GCATGTGATCATCTGCATAGTCCTCTCCTCTAACGGGAAACACCTCAGATTTGCATATAAAAAAGCACCC
TGGTGCTGAAATGAACCCCTTTCTTGAACATCAAAGCTGTCTCCCACAGCCTTGGGCAGCAGGGTGCCTC
TTAGTGGATGTGCTGGGTCCACCCTGAGCCCTGACATGTGGTGGCAGCATTGCCAGTTGGTCTGTGTGTC
TGTGTAGCAGGGACGATTTCCCAGAAAGCAATTTTCCTTTTGAAATACGTAATTGTTGAGACTAGGCAGT
TTCAAAGTCAGCTGCATATAGTAGCAAGTACAGGACTGTCTTGTTTTTGGTGTCCTTGGAGGTGCTGGGG
TGAGGGTTTCAGTGGGATCATTTACTCTCACATGTTGTCTGCCTTCTGCTTCTGTGGACACTGCTTTGTA
CTTAATTCAGACAGACTGTGAATACACCTTTTTTATAAATACCTTTCAAATTCTTGGTAAGATATAATTT
TGATAGCTGATTGCAGATTTTCTGTATTTGTCAGATTAATAAAGACTGCATGAATCCAAAAAAAAAAA
AAAAA
>NM 000447.2 Homo sapiens presenilin 2 (PSEN2), transcript variant 1, mRNA (SEQ ID NO:3) GGGGCCTGGGCCGGCGCCGGGTCCGGCCGGGCGCTCAGCCAGCTGCGTAAACTCCGCTGGAGCGCGGCGG
CAGAGCAGGCATTTCCAGCAGTGAGGAGACAGCCAGAAGCAAGCTTTTGGAGCTGAAGGAACCTGAGACA
GAAGCTAGTCCCCCCTCTGAATTTTACTGATGAAGAAACTGAGGCCACAGAGCTAAAGTGACTTTTCCCA
AGGTCGCCCAGCGAGGACGTGGGACTTCTCAGACGTCAGGAGAGTGATGTGAGGGAGCTGTGTGACCATA
GAAAGTGACGTGTTAAAAACCAGCGCTGCCCTCTTTGAAAGCCAGGGAGCATCATTCATTTAGCCTGCTG
AGAAGAAGAAACCAAGTGTCCGGGATTCAGACCTCTCTGCGGCCCCAAGTGTTCGTGGTGCTTCCAGAGG
CAGGGCTATGCTCACATTCATGGCCTCTGACAGCGAGGAAGAAGTGTGTGATGAGCGGACGTCCCTAATG
TCGGCTGAGAGCCCCACGCCGCGCTCCTGCCAGGAGGGCAGGCAGGGCCCAGAGGATGGAGAGAACACTG
CCCAGTGGAGAAGCCAGGAGAACGAGGAGGACGGTGAGGAGGACCCTGACCGCTATGTCTGTAGTGGGGT
TCCCGGGCGGCCGCCAGGCCTGGAGGAAGAGCTGACCCTCAAATACGGAGCGAAGCACGTGATCATGCTG
TTTGTGCCTGTCACTCTGTGCATGATCGTGGTGGTAGCCACCATCAAGTCTGTGCGCTTCTACACAGAGA
AGAATGGACAGCTCATCTACACGCCATTCACTGAGGACACACCCTCGGTGGGCCAGCGCCTCCTCAACTC
CGTGCTGAACACCCTCATCATGATCAGCGTCATCGTGGTTATGACCATCTTCTTGGTGGTGCTCTACAAG
TACCGCTGCTACAAGTTCATCCATGGCTGGTTGATCATGTCTTCACTGATGCTGCTGTTCCTCTTCACCT
ATATCTACCTTGGGGAAGTGCTCAAGACCTACAATGTGGCCATGGACTACCCCACCCTCTTGCTGACTGT
CTGGAACTTCGGGGCAGTGGGCATGGTGTGCATCCACTGGAAGGGCCCTCTGGTGCTGCAGCAGGCCTAC
CTCATCATGATCAGTGCGCTCATGGCCCTAGTGTTCATCAAGTACCTCCCAGAGTGGTCCGCGTGGGTCA
TCCTGGGCGCCATCTCTGTGTATGATCTCGTGGCTGTGCTGTGTCCCAAAGGGCCTCTGAGAATGCTGGT
AGAAACTGCCCAGGAGAGAAATGAGCCCATATTCCCTGCCCTGATATACTCATCTGCCATGGTGTGGACG
GTTGGCATGGCGAAGCTGGACCCCTCCTCTCAGGGTGCCCTCCAGCTCCCCTACGACCCGGAGATGGAAG
AAGACTCCTATGACAGTTTTGGGGAGCCTTCATACCCCGAAGTCTTTGAGCCTCCCTTGACTGGCTACCC
AGGGGAGGAGCTGGAGGAAGAGGAGGAAAGGGGCGTGAAGCTTGGCCTCGGGGACTTCATCTTCTACAGT
GTGCTGGTGGGCAAGGCGGCTGCCACGGGCAGCGGGGACTGGAATACCACGCTGGCCTGCTTCGTGGCCA
TCCTCATTGGCTTGTGTCTGACCCTCCTGCTGCTTGCTGTGTTCAAGAAGGCGCTGCCCGCCCTCCCCAT
CTCCATCACGTTCGGGCTCATCTTTTACTTCTCCACGGACAACCTGGTGCGGCCGTTCATGGACACCCTG
GCCTCCCATCAGCTCTACATCTGAGGGACATGGTGTGCCACAGGCTGCAAGCTGCAGGGAATTTTCATTG
GATGCAGTTGTATAGTTTTACACTCTAGTGCCATATATTTTTAAGACTTTTCTTTCCTTAAAAAATAAAG
TACGTGTTTACTTGGTGAGGAGGAGGCAGAACCAGCTCTTTGGTGCCAGCTGTTTCATCACCAGACTTTG
GCTCCCGCTTTGGGGAGCGCCTCGCTTCACGGACAGGAAGCACAGCAGGTTTATCCAGATGAACTGAGAA

GGTCAGATTAGGGCGGGGAGAAGAGCATCCGGCATGAGGGCTGAGATGCGCAAAGAGTGTGCTCGGGAGT
GGCCCCTGGCACCTGGGTGCTCTGGCTGGAGAGGAAAAGCCAGTTCCCTACGAGGAGTGTTCCCAATGCT
TTGTCCATGATGTCCTTGTTATTTTATTGCCTTTAGAAACTGAGTCCTGTTCTTGTTACGGCAGTCACAC
TGCTGGGAAGTGGCTTAATAGTAATATCAATAAATAGATGAGTCCTGTTAGAATCTTGAAAA
>NM 012486.2 Homo sapiens presenilin 2 (PSEN2), transcript variant 2, mRNA (SEQ ID NO:4) GGGGCCTGGGCCGGCGCCGGGTCCGGCCGGGCGCTCAGCCAGCTGCGTAAACTCCGCTGGAGCGCGGCGG
CAGAGCAGGCATTTCCAGCAGTGAGGAGACAGCCAGAAGCAAGCTTTTGGAGCTGAAGGAACCTGAGACA
GAAGCTAGTCCCCCCTCTGAATTTTACTGATGAAGAAACTGAGGCCACAGAGCTAAAGTGACTTTTCCCA
AGGTCGCCCAGCGAGGACGTGGGACTTCTCAGACGTCAGGAGAGTGATGTGAGGGAGCTGTGTGACCATA
GAAAGTGACGTGTTAAAAACCAGCGCTGCCCTCTTTGAAAGCCAGGGAGCATCATTCATTTAGCCTGCTG
AGAAGAAGAAACCAAGTGTCCGGGATTCAGACCTCTCTGCGGCCCCAAGTGTTCGTGGTGCTTCCAGAGG
CAGGGCTATGCTCACATTCATGGCCTCTGACAGCGAGGAAGAAGTGTGTGATGAGCGGACGTCCCTAATG
TCGGCTGAGAGCCCCACGCCGCGCTCCTGCCAGGAGGGCAGGCAGGGCCCAGAGGATGGAGAGAACACTG
CCCAGTGGAGAAGCCAGGAGAACGAGGAGGACGGTGAGGAGGACCCTGACCGCTATGTCTGTAGTGGGGT
TCCCGGGCGGCCGCCAGGCCTGGAGGAAGAGCTGACCCTCAAATACGGAGCGAAGCACGTGATCATGCTG
TTTGTGCCTGTCACTCTGTGCATGATCGTGGTGGTAGCCACCATCAAGTCTGTGCGCTTCTACACAGAGA
AGAATGGACAGCTCATCTACACGCCATTCACTGAGGACACACCCTCGGTGGGCCAGCGCCTCCTCAACTC
CGTGCTGAACACCCTCATCATGATCAGCGTCATCGTGGTTATGACCATCTTCTTGGTGGTGCTCTACAAG
TACCGCTGCTACAAGTTCATCCATGGCTGGTTGATCATGTCTTCACTGATGCTGCTGTTCCTCTTCACCT
ATATCTACCTTGGGGAAGTGCTCAAGACCTACAATGTGGCCATGGACTACCCCACCCTCTTGCTGACTGT
CTGGAACTTCGGGGCAGTGGGCATGGTGTGCATCCACTGGAAGGGCCCTCTGGTGCTGCAGCAGGCCTAC
CTCATCATGATCAGTGCGCTCATGGCCCTAGTGTTCATCAAGTACCTCCCAGAGTGGTCCGCGTGGGTCA
TCCTGGGCGCCATCTCTGTGTATGATCTCGTGGCTGTGCTGTGTCCCAAAGGGCCTCTGAGAATGCTGGT
AGAAACTGCCCAGGAGAGAAATGAGCCCATATTCCCTGCCCTGATATACTCATCTGCCATGGTGTGGACG
GTTGGCATGGCGAAGCTGGACCCCTCCTCTCAGGGTGCCCTCCAGCTCCCCTACGACCCGGAGATGGAAG
ACTCCTATGACAGTTTTGGGGAGCCTTCATACCCCGAAGTCTTTGAGCCTCCCTTGACTGGCTACCCAGG
GGAGGAGCTGGAGGAAGAGGAGGAAAGGGGCGTGAAGCTTGGCCTCGGGGACTTCATCTTCTACAGTGTG
CTGGTGGGCAAGGCGGCTGCCACGGGCAGCGGGGACTGGAATACCACGCTGGCCTGCTTCGTGGCCATCC
TCATTGGCTTGTGTCTGACCCTCCTGCTGCTTGCTGTGTTCAAGAAGGCGCTGCCCGCCCTCCCCATCTC
CATCACGTTCGGGCTCATCTTTTACTTCTCCACGGACAACCTGGTGCGGCCGTTCATGGACACCCTGGCC
TCCCATCAGCTCTACATCTGAGGGACATGGTGTGCCACAGGCTGCAAGCTGCAGGGAATTTTCATTGGAT
GCAGTTGTATAGTTTTACACTCTAGTGCCATATATTTTTAAGACTTTTCTTTCCTTAAAAAATAAAGTAC
GTGTTTACTTGGTGAGGAGGAGGCAGAACCAGCTCTTTGGTGCCAGCTGTTTCATCACCAGACTTTGGCT
CCCGCTTTGGGGAGCGCCTCGCTTCACGGACAGGAAGCACAGCAGGTTTATCCAGATGAACTGAGAAGGT
CAGATTAGGGCGGGGAGAAGAGCATCCGGCATGAGGGCTGAGATGCGCAAAGAGTGTGCTCGGGAGTGGC
CCCTGGCACCTGGGTGCTCTGGCTGGAGAGGAAAAGCCAGTTCCCTACGAGGAGTGTTCCCAATGCTTTG
TCCATGATGTCCTTGTTATTTTATTGCCTTTAGAAACTGAGTCCTGTTCTTGTTACGGCAGTCACACTGC
TGGGAAGTGGCTTAATAGTAATATCAATAAATAGATGAGTCCTGTTAGAATCTTGAAAA

>NP 000012.1 presenilin-1 isoform 1-467 [Homo sapiens] SEO ID NO:5) MTELPAPLSYFQNAQMSEDNHLSNIVRSQNDNRERQEHNDRRSLGHPEPLSNGRPQGNSRQVVEQ
DEE EDEELTLKYGAKHVIML FVPVTLCMVVVVAT I KSVS FYTRKDGQL I YT P FTE DT ETVGQRAL
HS ILNAAIMI SVIVVMT I LLVVLYKYRCYKVI HAWL I ISS LLLL FFFS F I YLGEVFKTYN
VAVDY I TVALL IWNFGVVGMI S I HWKGPLRLQQAYL IMI SALMALVF I KYL PEWTAWL I
LAVI SVYDLVAVLCPKGPLRMLVETAQERNETLFPAL I YS S TMVWLVNMAEGDPEAQRR
VSKNSKYNAES TERESQDTVAENDDGGFSEEWEAQRDSHLGPHRS T PE SRAAVQEL S S S
I LAGEDPEERGVKLGLGDF I FYSVLVGKASATASGDWNT T IACFVAIL I GLCLTLLLLA
I FKKAL PAL PIS IT FGLVFY FAT DYLVQP FMDQLAFHQFY I
>NP 015557.2 presenilin-1 isoform 1-463 [Homo sapiens](SEQ ID NO:6) MTELPAPLSYFQNAQMSEDNHLSNINDNRERQEHNDRRSLGHPEPLSNGRPQGNSRQVVEQDEEEDEE
LILKYGAKHVIMLFVPVTLCMVVVVATIKSVSFYIRKDGQLIYIPFTEDTETVGQRALHSILNAAIMI
SVIVVMTILLVVLYKYRCYKVIHAWLIISSLLLLFFFSFIYLGEVEKTYNVAVDYITVALLIWNFGVV
GMISIHWKGPLRLQQAYLIMISALMALVFIKYLPEWTAWLILAVISVYDLVAVLCPKGPLRMLVETAQ
ERNETLFPALIYSSTMVWLVNMAEGDPEAQRRVSKNSKYNAESTERESQDTVAENDDGGFSEEWEAQR
DSHLGPHRSTPESRAAVQELSSSILAGEDPEERGVKLGLGDFIFYSVLVGKASATASGDWNITIACFV
AILIGLCLILLLLAIFKKALPALPISITFGLVFYFAIDYLVQPFMDQLAFHQFYI
>NP 000438.2 presenilin-2 isoform 1 [Homo sapiens] (SEQ ID NO:7) MLIFMASDSEEEVCDERTSLMSAESPIPRSCQEGRQGPEDGENTAQWRSQENEEDGEEDPDRYVCSGV
PGRPPGLEEELTLKYGAKHVIMLFVPVTLCMIVVVATIKSVRFYTEKNGQLIYIPFTEDTPSVGQRLL
NSVLNTLIMISVIVVMTIFLVVLYKYRCYKFIHGWLIMSSLMLLFLFTYIYLGEVLKTYNVAMDYPIL
LLTVWNFGAVGMVCIHWKGPLVLQQAYLIMISALMALVFIKYLPEWSAWVILGAISVYDLVAVLCPKG
PLRMLVETAQERNEPIFPALIYSSAMVWTVGMAKLDPSSQGALQLPYDPEMEEDSYDSFGEPSYPEVF
EPPLIGYPGEELEEEEERGVKLGLGDFIFYSVLVGKAAATGSGDWNTTLACFVAILIGLCLILLLLAV
FKKALPALPISITFGLIFYFSTDNLVRPFMDTLASHQLYI
>NP 036618.2 presenilin-2 isoform 2 [Homo sapiens] (SEQ ID NO:8) MLIFMASDSEEEVCDERTSLMSAESPIPRSCQEGRQGPEDGENTAQWRSQENEEDGEEDPDRYVCSGV
PGRPPGLEEELTLKYGAKHVIMLFVPVTLCMIVVVATIKSVRFYTEKNGQLIYIPFTEDTPSVGQRLL
NSVLNTLIMISVIVVMTIFLVVLYKYRCYKFIHGWLIMSSLMLLFLFTYIYLGEVLKTYNVAMDYPIL
LLTVWNFGAVGMVCIHWKGPLVLQQAYLIMISALMALVFIKYLPEWSAWVILGAISVYDLVAVLCPKG
PLRMLVETAQERNEPIFPALIYSSAMVWTVGMAKLDPSSQGALQLPYDPEMEDSYDSFGEPSYPEVFE
PPLIGYPGEELEEEEERGVKLGLGDFIFYSVLVGKAAATGSGDWNTTLACFVAILIGLCLILLLLAVF
KKALPALPISITFGLIFYFSTDNLVRPFMDTLASHQLYI

To determine the percent identity of two amino acid sequences, or of two nucleic acid sequences, the sequences are aligned for optimal comparison purposes (e.g., gaps can be introduced in one or both of a first and a second amino acid or nucleic acid sequence for optimal alignment and non-homologous sequences can be disregarded for comparison purposes). The length of a reference sequence aligned for comparison purposes is at least 80% of the length of the reference sequence, and in some embodiments is at least 90% or 100%. The amino acid residues or nucleotides at corresponding amino acid positions or nucleotide positions are then compared. When a position in the first sequence is occupied by the same amino acid residue or nucleotide as the corresponding position in the second sequence, then the molecules are identical at that position. The percent identity between the two sequences is a function of the number of identical positions shared by the sequences, taking into account the number of gaps, and the length of each gap, which need to be introduced for optimal alignment of the two sequences. In another embodiment, the percent identity of two amino acid sequences can be assessed as a function of the conservation of amino acid residues within the same family of amino acids (e.g., positive charge, negative charge, polar and uncharged, hydrophobic) at corresponding positions in both amino acid sequences (e.g., the presence of an alanine residue in place of a valine residue at a specific position in both sequences shows a high level of conservation, but the presence of an arginine residue in place of an aspartate residue at a specific position in both sequences shows a low level of conservation).
For example, the percent identity between two amino acid sequences can be determined using the Needleman and Wunsch ((1970) J. Mol. Biol. 48:444-453 ) algorithm which has been incorporated into the GAP program in the GCG software package, using a Blossum scoring matrix, e.g., with default values for gap penalty, gap extend penalty of 4, and frameshift gap penalty.
Codon Optimized Presenilin 1 Codon optimization is desirable to express proteins in specific host cells ¨
e.g., bacterial, mouse, human. It will be appreciated by those skilled in the art that as a result of the degeneracy of the genetic code, a multitude of cDNAs encoding human presenilin 1, some bearing minimal similarity to the cDNAs of any known and naturally occurring gene, may be produced. Thus, the invention contemplates each and every possible variation of cDNA that could be made by selecting combinations based on possible codon choices. These combinations are made in accordance with the standard triplet genetic code as applied to the polynucleotide encoding naturally occurring human presenilin variant, and all such variations are to be considered as being specifically disclosed. An exemplary codon-optimized human PSEN1 nucleotide sequence is disclosed herein ¨ e.g., SEQ ID NO:9; See Fig. 2.
This codon-optimized human PSEN1 nucleotide sequence was generated by substituting codons in the naturally occurring PSEN1 nucleotide sequence that occur at lower frequency in human cells for codons that occur at higher frequency in human cells. Codon-optimized human PSEN1 nucleotide sequences can include sequences wherein less than 100% of the codons are optimized, e.g., wherein only 20%, 30%, 40%, 50%, 60%, 70%, 80%, or 90% of the wild type non-optimized codons are optimized. The frequency of occurrence for codons can be computationally determined by methods known in the art. An exemplary calculation of these codon frequencies is disclosed in Table 1.
An exemplary codon-optimized human PSEN1 sequence is as follows:
>Codon optimized Homo sapiens presenilin 1 (PSEN1) cDNA (SEQ ID
NO: 9) CGACGCCACCATGACAGAACTGCCIGCCCCCCTGAGCTACTICCAGAACGCCCAGATGAGCGAGGACA
ACCACCTGAGCAACACCGTGCGGAGCCAGAACGACAACAGAGAGCGGCAGGAACACAACGACAGGCGG
AGCCIGGGACACCCTGAGCCCCIGICTAATGGCAGACCCCAGGGCAACAGCAGACAGGIGGIGGAACA
GGACGAGGAAGAGGACGAAGAACTGACCCTGAAGTACGGCGCCAAGCACGTGATCATGCTGITCGTGC
CCGTGACCCTGTGCATGGTCGTGGTGGTGGCCACAATCAAGAGCGTGTCCTTCTACACCCGGAAGGAC
GGCCAGCTGATCTACACCCCCTTCACCGAGGACACCGAGACAGTGGGACAGAGAGCCCTGCACAGCAT
CCTGAACGCCGCCATCATGATCAGCGTGATCGTCGTGATGACCATCCTGCTGGTGGTGCTGTACAAGT
ACCGGIGCTACAAAGTGATCCACGCCIGGCTGATCATCAGCAGCCIGCTGCTGCTGITCTICITTAGC
TICATCTACCIGGGCGAGGIGTICAAGACCIACAACGIGGCCGIGGACTACATCACCGIGGCCCIGCT
GATCTGGAACTICGGCGICGTGGGCATGATCTCCATCCACTGGAAGGGCCCCCTGAGACTGCAGCAGG
CCTACCTGATTATGATCTCCGCCCTGATGGCCCTGGTGTTCATCAAGTACCTGCCCGAGTGGACCGCT
TGGCTGATCCTGGCCGTGATCTCCGTGTACGACCTGGTGGCCGTGCTGTGCCCTAAGGGACCTCTGCG
GATGCTGGIGGAAACCGCCCAGGAACGGAACGAGACACTGITCCCIGCCCTGATCTACTCCAGCACAA
TGGIGIGGCTCGTGAACATGGCCGAGGGCGATCCTGAGGCCCAGCGGAGAGIGICCAAGAACTCCAAG
TACAACGCCGAGAGCACCGAGCGCGAGAGCCAGGATACAGIGGCCGAGAATGACGACGGCGGCTICAG
CGAGGAATGGGAGGCCCAGAGAGATAGCCACCIGGGCCCICACAGAAGCACCCCTGAATCTAGAGCCG
CCGTGCAGGAACTGAGCAGCTCCATICIGGCCGGCGAGGACCCCGAAGAAAGAGGCGTGAAACTGGGC
CTGGGCGACTTCATCTTCTACAGCGTGCTCGTGGGCAAGGCCAGCGCCACAGCTAGCGGCGACTGGAA
CACCACAATCGCCTGCTTCGTGGCCATCCTGATCGGCCTGTGTCTGACACTTCTGCTGCTGGCCATCT
TCAAGAAGGCCCIGCCCGCCCIGCCIATCAGCATCACCITCGGCCIGGIGITTTACTICGCCACCGAC
TACCTGGTGCAGCCCTTCATGGACCAGCTGGCCTTCCACCAGTTCTACATCTGA

Table 1. Codon Usage Frequency Table in Humans (Source: Gen Script , GenScript Codon Usage Frequency Table Tool) Triplet Am Frequency/ino acid Fraction Number Thousand ITT F 0.45 16.9 336562 TIC F 0.55 20.4 406571 TTA L 0.07 7.2 143715 TTG L 0.13 12.6 249879 TAT Y 0.43 12 239268 TAC Y 0.57 15.6 310695 TAA * 0.28 0.7 14322 TAG * 0.2 0.5 10915 CTT L 0.13 12.8 253795 CTC L 0.2 19.4 386182 CIA L 0.07 6.9 138154 CTG L 0.41 40.3 800774 CAT H 0.41 10.4 207826 CAC H 0.59 14.9 297048 CAA 4 0.25 11.8 234785 CAG 4 0.75 34.6 688316 ATT I 0.36 15.7 313225 ATC I 0.48 21.4 426570 ATA I 0.16 7.1 140652 ATG M 1 22.3 443795 AAT N 0.46 16.7 331714 AAC N 0.54 19.5 387148 AAA K 0.42 24 476554 AAG K 0.58 32.9 654280 GTT V 0.18 10.9 216818 GTC V 0.24 14.6 290874 GTA V 0.11 7 139156 GIG V 0.47 28.9 575438 GAT D 0.46 22.3 443369 GAC D 0.54 26 517579 GAA E 0.42 29 577846 GAG E 0.58 40.8 810842 TCT s 0.18 14.6 291040 TCC s 0.22 17.4 346943 TCA s 0.15 11.7 233110 TCG s 0.06 4.5 89429 TGT C 0.45 9.9 197293 TGC C 0.55 12.2 243685 TGA * 0.52 1.3 25383 TGG W 1 12.8 255512 CCT P 0.28 17.3 343793 CCC P 0.33 20 397790 CCA P 0.27 16.7 331944 CCG P 0.11 7 139414 CGT R 0.08 4.7 93458 CGC R 0.19 10.9 217130 CGA R 0.11 6.3 126113 CGG R 0.21 11.9 235938 Triplet Am Frequency/ino acid Fraction Number Thousand ACT T 0.24 12.8 ACC T 0.36 19.2 ACA T 0.28 14.8 ACG T 0.12 6.2 AGT S 0.15 11.9 AGC S 0.24 19.4 AGA R 0.2 11.5 AGG R 0.2 11.4 GCT A 0.26 18.6 GCC A 0.4 28.5 GCA A 0.23 16 GCG A 0.11 7.6 GGT G 0.16 10.8 GGC G 0.34 22.8 GGA G 0.25 16.3 GGG G 0.25 16.4 Mutated Presenilin 1 In some embodiments, the PS1 protein contains a mutation. In some embodiments, the mutation is a conservative substitution. Such changes include substituting any of isoleucine (I), valine (V), and leucine (L) for any other of these hydrophobic amino acids;
aspartic acid (D) for glutamic acid (E) and vice versa; glutamine (Q) for asparagine (N) and vice versa; and serine (S) for threonine (T) and vice versa. Other substitutions can also be considered conservative, depending on the environment of the particular amino acid and its role in the three-dimensional structure of the protein. For example, glycine (G) and alanine (A) can frequently be interchangeable, as can alanine (A) and valine (V).
Methionine (M), which is relatively hydrophobic, can frequently be interchanged with leucine and isoleucine, and sometimes with valine. Lysine (K) and arginine (R) are frequently interchangeable in locations in which the significant feature of the amino acid residue is its charge and the differing pK's of these two amino acid residues are not significant. Still other changes can be considered "conservative" in particular environments (see, e.g. Table III of US20110201052;
pages 13-15 "Biochemistry" 2nd ED. Stryer ed (Stanford University); Henikoff et al., PNAS
1992 Vol 89 10915-10919; Lei et al., J Biol Chem 1995 May 19; 270(20):11882-6).
In some embodiments, the methods include introducing one or more additional mutations into the human PS1 sequence (SEQ ID NOs:5 or 6). Thus, in some embodiments, the sequence can be at least 80%, 85%, 90%, 95%, or 99% identical to at least 60%, 70%, 80%, 90%, or 100% of a human PS1.

To determine the percent identity of two amino acid sequences, or of two nucleic acid sequences, the sequences are aligned for optimal comparison purposes (e.g., gaps can be introduced in one or both of a first and a second amino acid or nucleic acid sequence for optimal alignment and non-homologous sequences can be disregarded for comparison purposes). The length of a reference sequence aligned for comparison purposes is typically at least 80% of the length of the reference sequence, and in some embodiments is at least 90%
or 100%. The amino acid residues or nucleotides at corresponding amino acid positions or nucleotide positions are then compared. When a position in the first sequence is occupied by the same amino acid residue or nucleotide as the corresponding position in the second sequence, then the molecules are identical at that position (as used herein amino acid or nucleic acid "identity" is equivalent to amino acid or nucleic acid "homology"). The percent identity between the two sequences is a function of the number of identical positions shared by the sequences, taking into account the number of gaps, and the length of each gap, which need to be introduced for optimal alignment of the two sequences. In another embodiment, the percent identity of two amino acid sequences can be assessed as a function of the conservation of amino acid residues within the same family of amino acids (e.g., positive charge, negative charge, polar and uncharged, hydrophobic) at corresponding positions in both amino acid sequences (e.g., the presence of an alanine residue in place of a valine residue at a specific position in both sequences shows a high level of conservation, but the presence of an arginine residue in place of an aspartate residue at a specific position in both sequences shows a low level of conservation).
For purposes of the present methods, the comparison of sequences and determination of percent identity between two sequences can be accomplished using a Blossum 62 scoring matrix with a gap penalty of 12, a gap extend penalty of 4, and a frameshift gap penalty of 5.
Delivery Vectors Codon-optimized nucleic acids encoding a PS1 polypeptide or therapeutically active fragment thereof can be incorporated into a gene construct to be used as a part of a gene therapy protocol. For example, described herein are targeted expression vectors for in vivo delivery and expression of a codon-optimized polynucleotide that encodes a PS1 polypeptide or active fragment thereof in particular cell types, especially cerebral cortical neuronal cells.
Expression constructs of such components can be administered in any effective carrier, e.g., any formulation or composition capable of effectively delivering the component gene to cells in vivo. Approaches include insertion of the gene in viral vectors, preferably adeno-associated virus. Viral vectors typically transduce cells directly.
Viral vectors capable of highly efficient transduction of CNS neurons may be employed, including any serotypes of rAAV (e.g., AAV1-AAV12) vectors, recombinant or chimeric AAV vectors, as well as lentivirus or other suitable viral vectors.
In some embodiments, a codon-optimized polynucleotide encoding PS1 is operably linked to promoter suitable for expression in the CNS. For example, a neuron subtype-specific specific promoter, such as the alpha-calcium/calmodulin kinase 2A promoter may be used to target excitatory neurons. Alternatively, a pan neuronal promoter, such as the synapsin I promoter, may be used to drive PS1 expression. Other exemplary promoters include, but are not limited to, a cytomegalovirus (CMV) early enhancer/promoter; a hybrid CMV
enhance/chicken (3-actin (CBA) promoter; a promoter comprising the CMV early enhancer element, the first exon and first intron of the chicken 13-actin gene, and the splice acceptor of the rabbit 13-globin gene (commonly call the "CAG promoter"); or a 1.6-kb hybrid promoter composed of a CMV immediate-early enhancer and CBA intron l/exon 1 (commonly called the CAGGS
promoter; Niwa et al. Gene, 108:193-199 (1991)). The CAGGS promoter (Niwa et al., 1991) has been shown to provide ubiquitous and long-term expression in the brain (Klein et al., Exp. Neurol. 176:66-74 (2002)). One approach for in vivo introduction of nucleic acid into a cell is by use of a viral vector containing nucleic acid, e.g., a codon-optimized cDNA
encoding a PS1. Among other things, infection of cells with a viral vector has the advantage that a large proportion of the targeted cells can receive the nucleic acid.
Additionally, molecules encoded within the viral vector, e.g., by a cDNA contained in the viral vector, are expressed efficiently in cells that have taken up viral vector nucleic acid.
A viral vector system particularly useful for delivery of nucleic acids is the adeno-associated virus (AAV). Adeno-associated virus is a naturally occurring defective virus that requires another virus, such as an adenovirus or a herpes virus, as a helper virus for efficient replication and a productive life cycle. (For a review see Muzyczka et al., Curr. Topics in Micro and Immuno1.158:97-129 (1992)). AAV vectors efficiently transduce various cell types and can produce long-term expression of transgenes in vivo. Although AAV
vector genomes can persist within cells as episomes, vector integration has been observed (see for example Deyle and Russell, Curr Opin Mol Ther. 2009 Aug; 11(4): 442-447;
Asokan et al., Mol Ther. 2012 April; 20(4): 699-708; Flotte et al., Am. J. Respir. Cell. Mol.
Biol. 7:349-356 (1992); Samulski et al., J. Virol. 63:3822-3828 (1989); and McLaughlin et al., J. Virol.
62:1963-1973 (1989)). AAV vectors, such as AAV2, have been extensively used for gene augmentation or replacement and have shown therapeutic efficacy in a range of animal models as well as in the clinic; see, e.g., Mingozzi and High, Nature Reviews Genetics 12, 341-355 (2011); Deyle and Russell, Curr Opin Mol Ther. 2009 Aug; 11(4): 442-447; Asokan et al., Mol Ther. 2012 April; 20(4): 699-708. AAV vectors containing as little as 300 base pairs of AAV can be packaged and can produce recombinant protein expression.
Protocols for producing recombinant retroviruses and for infecting cells in vitro or in vivo with such viruses are known in the art, e.g, can be found in Ausubel, et al., eds., Current Protocols in Molecular Biology, Greene Publishing Associates, (1989), Sections 9.10-9.14, and other standard laboratory manuals. The use of AAV vectors to deliver constructs for expression in the brain has been described, e.g., in Iwata et al., Sci Rep. 2013;3:1472;
Hester et al., Curr Gene Ther. 2009 Oct;9(5):428-33; Doll et al., Gene Therapy 1996, 3(5):437-447;
and Foley et al., J Control Release. 2014 Dec 28;196:71-8.
Thus, in some embodiments, the codon-optimized PSENlencoding nucleic acid is present in a vector for gene therapy, such as an AAV vector. In some instances, the AAV
vector is selected from the group consisting of AAV1, AAV2, AAV3, AAV4, AAV5, AAV6, AAV7, AAV8, AAV9, AAVrh10, AAV11, and AAV12. In preferred embodiments, the AAV

is AAV9 or AAVrh10.
A vector as described herein can be a pseudotyped vector. Pseudotyping provides a mechanism for modulating a vector's target cell population. For instance, pseudotyped AAV
vectors can be utilized in various methods described herein. Pseudotyped vectors are those that contain the genome of one vector, e.g., the genome of one AAV serotype, in the capsid of a second vector, e.g., a second AAV serotype. Methods of pseudotyping are well known in the art. For instance, a vector may be pseudotyped with envelope glycoproteins derived from Rhabdovirus vesicular stomatitis virus (VSV) serotypes (Indiana and Chandipura strains), rabies virus (e.g., various Evelyn¨Rokitnicki¨Abelseth ERA strains and challenge virus standard (CVS)), Lyssavirus Mokola virus, a rabies-related virus, vesicular stomatitis virus (VSV), Mokola virus (MV), lymphocytic choriomeningitis virus (LCMV), rabies virus glycoprotein (RV-G), glycoprotein B type (FuG-B), a variant of FuG-B (FuG-B2) or Moloney murine leukemia virus (MuLV). A virus may be pseudotyped for transduction of one or more neurons or groups of cells.
Without limitation, illustrative examples of pseudotyped vectors include recombinant AAV2/1, AAV2/2, AAV2/5, AAV2/6, AAV2/7, AAV2/8, AAV9, AAVrh10, AAV11, and AAV12 serotype vectors. It is known in the art that such vectors may be engineered to include a transgene encoding a human protein or other protein. In particular instances, the present disclosures can include a pseudotyped AAV9 or AAVrh10 viral vector including a nucleic acid as disclosed herein. See Viral Vectors for Gene Therapy: Methods and Protocols, ed. Machida, Humana Press, 2003.
In some instances, a particular AAV serotype vector may be selected based upon the intended use, e.g., based upon the intended route of administration.
Various methods for application of AAV vector constructs in gene therapy are known in the art, including methods of modification, purification, and preparation for administration to human subjects (see, e.g., Viral Vectors for Gene Therapy: Methods and Protocols, ed.
Machida, Humana Press, 2003). In addition, AAV based gene therapy targeted to cells of the CNS has been described (see, e.g., U.S. patents 6,180,613 and 6,503,888). High titer AAV
preparations can be produced using techniques known in the art, e.g., as described in U.S.
Pat. No. 5,658,776 A vector construct refers to a polynucleotide molecule including all or a portion of a viral genome and a transgene. In some instances, gene transfer can be mediated by a DNA
viral vector, such as an adenovirus (Ad) or adeno-associated virus (AAV).
Other vectors useful in methods of gene therapy are known in the art. For example, a construct as disclosed herein can include an alphavirus, herpesvirus, retrovirus, lentivirus, or vaccinia virus.
Adenoviruses are a relatively well characterized group of viruses, including over 50 serotypes (see, e.g., WO 95/27071, which is herein incorporated by reference).
Adenoviruses are tractable through the application of techniques of molecular biology and may not require integration into the host cell genome. Recombinant Ad-derived vectors, including vectors that reduce the potential for recombination and generation of wild-type virus, have been constructed (see, e.g., international patent publications WO 95/00655 and WO
95/11984, which are herein incorporated by reference). Wild-type AAV has high infectivity and is capable of integrating into a host genome with a high degree of specificity (see, e.g.
Hermonat and Muzyczka 1984 Proc. Natl. Acad. Sci., USA 81:6466-6470 and Lebkowski et al. 1988 Mol. Cell. Biol. 8:3988-3996).
Non-native regulatory sequences, gene control sequences, promoters, non-coding sequences, introns, or coding sequences can be included in a nucleic acid as disclosed herein.
The inclusion of nucleic acid tags or signaling sequences, or nucleic acids encoding protein tags or protein signaling sequences, is further contemplated herein.
Typically, the coding region is operably linked with one or more regulatory nucleic acid components.
A promoter included in a nucleic acid as disclosed herein can be a tissue- or cell type-specific promoter, a promoter specific to multiple tissues or cell types, an organ-specific promoter, a promoter specific to multiple organs, a systemic or ubiquitous promoter, or a nearly systemic or ubiquitous promoter. Promoters having stochastic expression, inducible expression, conditional expression, or otherwise discontinuous, inconstant, or unpredictable expression are also included within the scope of the present disclosure. A
promoter can include any of the above characteristics or other promoter characteristics known in the art.
In clinical settings, the gene delivery systems for the therapeutic gene can be introduced into a subject by any of a number of methods, each of which is familiar in the art.
For instance, a pharmaceutical preparation of the gene delivery system can be introduced systemically, e.g., by intravenous injection, and specific transduction of the protein in the target cells will occur predominantly from specificity of transfection, provided by the gene delivery vehicle, cell-type or tissue-type expression due to the transcriptional regulatory sequences controlling expression of the receptor gene, or a combination thereof In other embodiments, initial delivery of the recombinant gene is more limited, with introduction into the subject being quite localized. For example, the gene delivery vehicle can be introduced by catheter (see U.S. Patent 5,328,470) or by stereotactic injection, e.g., optionally into the cisterna magna, cerebral ventricles, lumbar intrathecal space, direct injection into hippocampus (e.g., Chen et al., PNAS USA 91: 3054-3057 (1994)). In preferred embodiments, delivery methods of Presenilin-expressing virus include intravenous, intrathecal, intracerebroventricular, intraci sternal, and stereotactic intraparenchymal administration.
The methods can be further optimized via preclinical testing to achieve the best rescue of neurodegeneration, dementia, synaptic dysfunction and molecular alteration in presenilin conditional double knockout mice and presenilin-1 knockin mice expressing FAD
mutations.
The pharmaceutical preparation of the gene therapy construct can consist essentially of the gene delivery system in an acceptable diluent, or can comprise a slow release matrix in which the gene delivery vehicle is embedded. Alternatively, where the complete gene delivery system can be produced intact from recombinant cells, e.g., retroviral vectors, the pharmaceutical preparation can comprise one or more cells, which produce the gene delivery system.
Delivery Formulations and Pharmaceutical Compositions In some embodiments, polynucleotides as disclosed herein for delivery to a target tissue in vivo are encapsulated or associated with in a nanoparticle. Methods for nanoparticle packaging are well known in the art, and are described, for example, in Bose S, et al (Role of Nucleolin in Human Parainfluenza Virus Type 3 Infection of Human Lung Epithelial Cells. J.
Virol. 78:8146. 2004); Dong Y et al. Poly(d,l-lactide-co-glycolide)/montmorillonite nanoparticles for oral delivery of anticancer drugs. Biomaterials 26:6068.
2005); Lobenberg R. et al (Improved body distribution of 14C-labelled AZT bound to nanoparticles in rats determined by radioluminography. J Drug Target 5:171.1998); Sakuma S R et al (Mucoadhesion of polystyrene nanoparticles having surface hydrophilic polymeric chains in the gastrointestinal tract. Int J Pharm 177:161. 1999); Virovic L et al. Novel delivery methods for treatment of viral hepatitis: an update. Expert Opin Drug Deliv 2:707.2005); and Zimmermann E et al, Electrolyte- and pH-stabilities of aqueous solid lipid nanoparticle (SLN) dispersions in artificial gastrointestinal media. Eur J Pharm Biopharm 52:203. 2001).
In some embodiments, one or more polynucleotides is delivered to a target tissue in vivo in a vesicle, e.g. a liposome (see Langer, Science 249:1527-1533 (1990); Treat et al., in Liposomes in the Therapy of Infectious Disease and Cancer, Lopez-Berestein and Fidler (eds.), Liss, New York, pp. 353-365 (1989); Lopez-Berestein, ibid., pp. 317-327; see generally ibid). In some embodiments, lipid-based nanoparticles (LNP) are used; see, e.g., Robinson et al., Mol Ther. 2018 Aug 1;26(8):2034-2046; U59956271B2.
The present methods and compositions can include microvesicles or a preparation thereof, that contains one or more therapeutic molecules ¨ e.g., polynucleotides or RNA ¨
described herein. "Microvesicles", as the term is used herein, refers to membrane-derived microvesicles, which includes a range of extracellular vesicles, including exosomes, microparticles and shed microvesicles secreted by many cell types under both normal physiological and pathological conditions. See, e.g., EP2010663B1. The methods and compositions described herein can be applied to microvesicles of all sizes; in one embodiment, 30 to 200 nm, in one embodiment, 30 to 800 nm, in one embodiment, up to 2 um. The methods and compositions described herein can also be more broadly applied to all extracellular vesicles, a term which encompasses exosomes, shed microvesicles, oncosomes, ectosomes, and retroviral-like particles. Such a microvesicle or preparation is produced by the herein described methods. As the term is used herein, a microvesicle preparation refers to a population of microvesicles obtained/prepared from the same cellular source.
Such a preparation is generated, for example, in vitro, by culturing cells expressing the nucleic acid molecule of the instant invention and isolating microvesicles produced by the cells. Methods of isolating such microvesicles are known in the art (Thery et al., Isolation and characterization of exosomes from cell culture supernatants and biological fluids, in Current Protocols Cell Biology, Chapter 3, 322, (John Wiley, 2006); Palmisano et al., (Mol Cell Proteomics. 2012 August; 11(8):230-43) and Waldenstrom et al., ((2012) PLoS
ONE 7(4):
e34653.doi: 10.1371/j ournal.pone.0034653)), some examples of which are described herein.
Such techniques for isolating microvesicles from cells in culture include, without limitation, sucrose gradient purification/separation and differential centrifugation, and can be adapted for use in a method or composition described herein. See, e.g., EP2010663B1.
In some embodiments, the microvesicles are isolated by gentle centrifugation (e.g., at about 300 g) of the culture medium of the donor cells for a period of time adequate to separate cells from the medium (e.g., about 15 minutes). This leaves the microvesicles in the supernatant, to thereby yield the microvesicle preparation. In one embodiment, the culture medium or the supernatant from the gentle centrifugation, is more strongly centrifuged (e.g., at about 16,000 g) for a period of time adequate to precipitate cellular debris (e.g., about 30 minutes). This leaves the microvesicles in the supernatant, to thereby yield the microvesicle preparation. In one embodiment, the culture medium, the gentle centrifuged preparation, or the strongly centrifuged preparation is subjected to filtration (e.g., through a 0.22 um filter or a 0.8 um filter, whereby the microvesicles pass through the filter. In one embodiment, the filtrate is subjected to a final ultracentrifugation (e.g. at about 110,000 g) for a period of time that will adequately precipitate the microvesicles (e.g. for about 80 minutes). The resulting pellet contains the microvesicles and can be resuspended in a volume of buffer that yields a useful concentration for further use, to thereby yield the microvesicle preparation. In one embodiment, the microvesicle preparation is produced by sucrose density gradient purification. In one embodiment, the microvesicles are further treated with DNAse (e.g., DNAse I) and/or RNAse and/or proteinase to eliminate any contaminating DNA, RNA, or protein, respectively, from the exterior. In one embodiment, the microvesicle preparation contains one or more RNAse inhibitors.
The molecules contained within the microvesicle preparation will comprise the therapeutic molecule. Typically the microvesicles in a preparation will be a heterogeneous population, and each microvesicle will contain a complement of molecule that may or may not differ from that of other microvesicles in the preparation. The content of the therapeutic molecules in a microvesicle preparation can be expressed either quantitatively or qualitatively. One such method is to express the content as the percentage of total molecules within the microvesicle preparation. By way of example, if the therapeutic molecule is an mRNA, the content can be expressed as the percentage of total RNA content, or alternatively as the percentage of total mRNA content, of the microvesicle preparation.
Similarly, if the therapeutic molecule is a protein, the content can be expressed as the percentage of total protein within the microvesicles. In one embodiment, therapeutic microvesicles, or a preparation thereof, produced by the method described herein contain a detectable, statistically significantly increased amount of the therapeutic molecule as compared to microvesicles obtained from control cells (cells obtained from the same source which have not undergone scientific manipulation to increase expression of the therapeutic molecule). In one embodiment, the therapeutic molecule is present in an amount that is at least about 10%, 20%, 30% 40%, 50%, 60%, 70% 80% or 90%, more than in microvesicles obtained from control cells. Higher levels of enrichment may also be achieved. In one embodiment, the therapeutic molecule is present in the microvesicle or preparation thereof, at least 2 fold more than control cell microvesicles. Higher fold enrichment may also be obtained (e.g., 3, 4, 5, 6, 7, 8, 9 or 10 fold).
In one embodiment, a relatively high percentage of the microvesicle content is the therapeutic molecule (e.g., achieved through overexpression or specific targeting of the molecule to microvesicles). In one embodiment, the microvesicle content of the therapeutic molecule is at least about 10%, 20%, 30% 40%, 50%, 60%, 70% 80% or 90%, of the total (like) molecule content (e.g., the therapeutic molecule is an mRNA and is about 10% of the total mRNA content of the microvesicle). Higher levels of enrichment may also be achieved.
In one embodiment, the therapeutic molecule is present in the microvesicle or preparation thereof, at least 2 fold more than all other such (like) molecules. Higher fold enrichment may also be obtained (e.g., 3, 4, 5, 6, 7, 8, 9 or 10 fold).
EXAMPLES
The invention is further described in the following examples, which do not limit the scope of the invention described in the claims.
Example 1: Dose-dependent rescue of y-secretase activity in MEFs with varying PS
genotypes: PS/+/+, pg/L435F/+, pg/L435F/ L435F, PS1 and PSP-; PS2-/-To determine whether reduced y-secretase activity associated with PSEN1 mutations can be corrected by introduction of wild-type (WT) hPS1, primary MEFs from embryos carrying varying PS genotypes, PS/+, p5iL435F/+, p5j+1-, p5iL435F/ L435F, ,-/-and PS/-/-;
PS2-/- (DKO) were derived. The immortalized MEFs were transiently transfected with CMV-NiE, and y-secretase activity was evaluated by measuring the levels of NICD
and PS1 NTF/CTF. The NICD levels were reduced in a PS1 dosage sensitive manner, and were undetectable in DKO cells (FIG. IA). The NICD levels were reduced but detectable in ps1L435F/ L435F MEFs ("L435F KI/KI" MEFs) and PS1-1" MEFs (FIG. IA), whereas de novo NICD production was undetectable by in vitro y-secretase assay using L435F
KI/KI and PSI"
I" embryonic brains (Xia et al., Neuron. 2015 Mar 4;85(5):967-81). Without wishing to be bound to a particular theory, applicant submits that this may be due to lower levels of PS2 normally expressed in the embryonic brain relative to MEFs, leading to lower overall PS
activity in L435F KI/KI and PS1-1" brains, relative to MEFs. To test this hypothesis, the y-secretase activity was measured in PS1L435F7+; p MEFs and compared to PS/L435 MEFs.
The y-secretase activity was lower in PS1L435F7+; p3"2-1- MEFs compared to PS/L435 MEFs (FIG. IB).
To determine whether the impaired y-secretase activity in various PS mutant MEFs can be rescued by introduction of WT hPS1, varying amounts (0, 20, 40, 80ng) of wild-type hPS1 cDNA (pCI-hPS1) were transfected into MEFs, along with CMV-NdE. Notably, increasing amounts ofpC1-hPS1 transfected into the MEFs resulted in accumulation of PS1 protein and restored levels of PS1 NTF and NICD in mutant (PS] L435, p5iL435F/+; PS2' --and DKO) MEFs (FIG. IB). These results indicate that exogenous WT hPS1 can rescue the impaired y-secretase activity in in various PS mutant MEFs.
Example 2: Development of an optimized wild-type human PSI in vitro expression system Methods Cell culture and transfection P sen-null mouse embryo fibroblasts (MEFs) lacking endogenous PS1 and PS2 were maintained in DMEM supplemented with 10% FBS and transiently transfected with plasmids expressing either the wild-type endogenous hPSEN1 cDNA (wt PS1) or the codon optimized hPSEN1 cDNA (opti PS1), with or without the y-secretase reporter, CMV-NdE, using Lipofectamine 3000 according to instruction. Cell lysates were collected at 24 h time point.
Western blotting Cell lysates were subjected to SDS-PAGE, and proteins were transferred to nitrocellulose membranes. After blocking in TBST/5% non-fat dry milk, membranes were incubated .. overnight with primary antibodies. To control for loading, membranes were stripped and re-probed with anti-P.-actin antibody. Band intensity was quantified using ImageJ
software, and results were normalized to 13-actin levels. Antibodies used included rat anti-PS1-NTF, rabbit anti-cleaved Notch (Va11744) (NICD), and mouse anti-P.-actin.
Results First, we expressed wt hPS1 or opti hPS1 in Psen-null MEFs to eliminate any contribution of endogenous PS1 or PS2. We detected a progressive increase in the levels of PS1 NTF when Psen-null MEFs were transfected with increasing amounts of vector encoding hPS1 or opti hPS1. Optimized hPS1 consistently expressed more PS1 relative to hP S1 (FIGs. 3A-3B).
NotchAE as substrate for y-secretase-mediated cleavage was co-expressed with wt hPS1 or opti hPS1 to measure y-secretase activity directly. Notch is cleaved by y-secretase to release the Notch intracellular domain (NICD). We evaluated the dose-response relationships for y-secretase-mediated cleavage of NotchAE to produce NICD as a function of y-secretase activity. Production of NICD increased linearly across the lower amounts of PS1 vectors transfected, but close to saturation at higher levels. More importantly, for each point, optimized hPS1 has higher y-secretase activity (FIG. 3).
Secreted endogenous A1340 and 42 levels are measured in the medium using ELISA.
Another y-secretase substrate, APP C99, is used to evaluate y-secretase activity by transiently transfecting CMV-C99 into each of the MEF cell lines, along with increasing amounts of pCI-hPSlopti. Primary and immortalized C410Y, E280A and D385A KU+ and KUKI
MEFs as well as PS1 KU+; PS2-/- MEFs are established. Whether KU+ and KUKI MEFs recapitulate similar phenotypes as KU+ and KUKI brains is determined, and whether introduction of WT hPS1 can restore the reduced y-secretase activity in a dose-dependent manner is measured by NICD and AICD production. The experiment is repeated with multiple independent MEF cell lines per genotype. Power analysis is performed to determine the sample size and the number of independent experiments needed to complete the study.
Example 3: Development of an optimized wild-type human PSI in vivo expression system Transgenic mice are developed that express human PSEN1 wild-type cDNA
constitutively or inducibly under the control of the CAMK2A promoter. To maximize PS1 production and activity, hPS1 was codon-optimized (hPSlopti), and then PS1 levels and y-secretase activity were compared between the endogenous hPS1 and hPSlopti cDNA
by co-transfecting increasing amounts of either pCI-hPS1 or pCI-hPSlopti and CMV-NAE
into PS
DKO MEFs. Relative to the endogenous hPS1 cDNA, the hPSlopti cDNA resulted in higher levels of PS1 NTF and higher y-secretase activity, measured by NICD production (FIG. 3).
Example 4: Determine whether postnatal delivery of hPSlopti can rescue phenotypes in PS cDKO mice The vectors listed in Table 2 have been prepared. The vector that confers the highest GFP staining at 4 and 8 weeks after injection is identified. To do this, PS
cDKO pups (lots ¨
breeding cages of F/F; -/-; Cre/Cre crossed with F/F; -/-) are injected at P0-2.
Table 2. List of vectors UID Description 01 AAV9/mCaMKII-intron-hPSlopti-T2A-EGFP-SV40pA
02 AAV9/hCaMKII-intron-hPSlopti-T2A-EGFP-SV40pA
03 AAV9/hCaMKII-intron- EGFP-SV40pA
04 AAV9/hSynI-intron-hPS1opti-T2A-EGFP-SV40pA
05 AAV9/hCaMKII-intron-hPS1opti-SV40pA
06 AAV9/hSynI-intron-hPS1opti-SV40A

10 An AAV ¨ e.g., AAV9/hCaMKII-intron-hPSlopti-T2A-EGFP-SV40pA or AAV9/hCaMKII-intron- EGFP-SV40pA ¨ is selected and injected into PS cDKO mice at P0-P2 by ICV. Western analysis is performed at 4 and 8 weeks of age to determine levels of PS1, APP, Nicastrin, PEN-2; control and PS cDKO mice are included at 4 and 8 weeks as additional controls. Gamma secretase activity, NICD production, and AP levels (by ELISA
of cortical lysates) are measured at 8 weeks of age. Additionally, at 2 months of age electrophysiological analysis ¨ e.g., Schaffer collateral, PPF, FF, and LTP ¨
is performed, and behavioral analysis is performed at 2-3 months of age ¨ e.g., watermaze.
Neuropath analysis is performed at 6 months of age.
Example 5: Determine whether postnatal delivery of hPSlopti can rescue phenotypes caused by FAD mutations Mice listed in Table 3 are generated, and analyzed using western blot analysis to measure PS1 and APP levels; in vitro gamma-secretase activity assay; ELISA, electrophysiological analysis at 6 months of age; behavior analysis at 6 and 12 months of age;
a neuropath analysis at 6, 12, and 18 months of age.

Table 3. List of mice genotypes Genotype Description of mice mated to generate the genotype PS1 L435F KU+ (C410Y KU+, from KU+ crossed with +/+: use KU+
E280A/E280A; -/-) PS1 L435F KU+; PS2-/- from KU+; -/- intercross: use KU+; -/-PS1 L435F KIMPS1; PS2-/-; CaM-Cre from KI/F; -/- crossed with KUF; -/-; Cre Example 6: Determine whether AAV9/hPSlopti delivered in the adult brain can rescue phenotypes caused by loss of PS function (PS cDKO, FAD KI) in vivo Vectors are prepared as listed in Table 2 and injected into mice either via intra-CSF, via ICM using 50u1 Hamilton syringe to deliver a lOul injection into the cisterna magna lx1012vg), via intraparenchymal delivery, or via intrathecal delivery using lOul 3.3 x1011vg lumber puncture. The mice studied will include (i) PS cDKO; (ii)KU+; (iii) KU+; P52-/-; and (iv)KUfPS1; P52-/-; Cre. We will perform the following analysis on the mice:
Western analysis to measure PS1 and APP levels; in vitro y-secretase assay; ELISA
measurements of A13 peptides, electrophysiological analysis at 6 months of age; behavior analysis at 6 and 12 months of age; a neuropath analysis at 6, 12, and 18 months of age.
OTHER EMBODIMENTS
It is to be understood that while the invention has been described in conjunction with the detailed description thereof, the foregoing description is intended to illustrate and not limit the scope of the invention, which is defined by the scope of the appended claims. Other aspects, advantages, and modifications are within the scope of the following claims.

Claims (23)

WHAT IS CLAIMED IS:

1. A composition comprising a human codon-optimized polynucleotide encoding a human presenilin 1 (PSEN1).

2. The composition of claim 1, wherein the human codon-optimized polynucleotide encoding a human PSEN1 is at least 95% identical to SEQ ID NO:9, with at least one codon optimized with respect to wild type.

3. The composition claim 1, wherein the human codon-optimized polynucleotide encoding a human PSEN1 comprises SEQ ID NO:9.

4. The composition of claims 1-3, which is associated with (e.g., formulated for delivery using) an exosome or lipid-based nanoparticle (LNP).

5. A composition comprising a vector for expression of human PSEN1 in a cell, comprising the human codon-optimized polynucleotide of claims 1-3, operably linked to a promoter.

6. The composition of claim 5, wherein the vector is a viral vector.

7. The composition of claim 6, wherein the viral vector is an adeno-associated viral (AAV) vector.

8. The composition of claim 7, wherein the AAV vector is AAV9 or AAVrh10.

9. The composition of claim 6, wherein the viral vector is a lentiviral vector or a retroviral vector.

10. The composition of claim 5, wherein the promoter is a pan neuronal promoter.

11. The composition of claim 10, wherein the pan neuronal promoter is a synapsin I
promoter.

12. The composition of claim 5, wherein the promoter is a neuron subtype-specific promoter.

13. The composition of claim 12, wherein the neuron subtype-specific promoter is an alpha-calcium/calmodulin kinase 2A promoter.

14. A method of treating a neurodegenerative disease, disorder, or condition, the method comprising administering to a human subject in need of treatment a composition of claims 1-13, wherein the subject has one or more mutations in at least one allele of PSEN1, preferably a mutation that encodes a dominant negative PSEN1 protein isoform.

15. The method of claim 14, wherein the neurodegenerative disease, disorder or condition is Alzheimer's disease.

16. The method of claim 15, wherein the Alzheimer's disease is familial Alzheimer's disease.

17. The method of claims 15 or 16, wherein the subject has a E280A, Y115H, L166P, C410Y, Aex9, G548, D257A, R278I, L435F, G384A, or L392Vmutation in the PSEN1 gene, or a N141I, G206A, H163R, A79V, 5290C, A260P, A426P, A431E, R269H, L271V, C1410Y, E280G, P264L, E185D, L235V, or M146V mutation in the PSEN1 gene.

18. The method of claim 15, wherein the Alzheimer's disease is sporadic Alzheimer's disease.

19. The method of claim 15, wherein the Alzheimer's disease is late-onset or early-onset Alzheimer's disease.

20. The method of claim 14, wherein the neurodegenerative disease, disorder or condition is frontotemporal dementia, memory loss, cognitive decline or impairment.

21. The method of claim 20, wherein the cognitive impairment is mild cognitive impairment (MCI).

22. The method of any one of claims 14-20, wherein the composition is administered to the CNS of the subject in need of treatment.

23. The method of claim 22, wherein the polynucleotide encoding PSEN1 and/or gene or mRNA is administered to the CNS via intravenous delivery, via intrathecal delivery, via intracisternal delivery, via intracerebroventricular delivery, or via stereotactic injection into certain areas of the brain, optionally into cisterna magna, cerebral ventricles, or lumbar intrathecal space, or via direct injection into hippocampus or cortical areas.